Cannabinoid Properties of Methylfluorophosphonate Analogs

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Martin, B. R.
	Articles by Razdan, R. K.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Martin, B. R.
	Articles by Razdan, R. K.

Vol. 294, Issue 3, 1209-1218, September 2000

Cannabinoid Properties of Methylfluorophosphonate Analogs¹

Billy R. Martin, Irina Beletskaya, Gray Patrick, Reneé Jefferson, Ramona Winckler, Dale G. Deutsch, Vincenzo Di Marzo, Olivier Dasse, Ann Mahadevan and Raj K. Razdan

Department of Pharmacology and Toxicology, Medical College of Virginia, Virginia Commonwealth University, Richmond, Virginia (B.R.M., I.B., G.P., R.J., R.W.); Department of Biochemistry and Cell Biology, State University of New York at Stony Brook, Stony Brook, New York (D.D.); Istituto per la Chimica di Molecole di Interesse Biologico, Napoli, Italy (V.D.M.); and Organix, Inc., Woburn, Massachusetts (O.D., A.M., R.K.R.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

Methylarachidonylfluorophosphonate (MAFP) and related analogs have been shown to inhibit fatty acid amidohydrolase activity(FAAH), the enzyme responsible for hydrolysis of the endogenouscannabinoid ligand anandamide. To fully characterize this classof compounds, methylfluorophosphonate compounds with saturatedalkyl chains ranging from C8 to C20 along with C20 unsaturatedderivatives were synthesized and evaluated for their ability tointeract with the CB1 receptor, inhibit FAAH, and produce in vivopharmacological effects. These analogs demonstrated widely varyingaffinities for the CB1 receptor. Of the saturated compounds, C8:0was incapable of displacing [³H]CP 55,940 binding, whereas C12:0 exhibited high affinity (2.5nM). The C20:0 saturated analog had low affinity (900 nM), butthe introduction of unsaturation into the C20 analogs restoredreceptor affinity. However, none of the analogs were capable offully displacing [³H]CP 55,940 binding. On the other hand, all compounds were ableto completely inhibit FAAH enzyme activity, with the C20:0 analogbeing the least potent. The most potent FAAH inhibitor was theshort-chained saturated C12:0, whereas the other analogs were15- to 30-fold less potent. In vivo, the C8:0 and C12:0 analogswere highly potent and fully efficacious in producing tetrahydrocannabinol(THC)-like effects, whereas the other analogs were either inactiveor acted as partial agonists. None was capable of attenuatingthe agonist effects of THC. Conversely, the C20:0 analog potentiatedthe effects of anandamide but not those of 2-arachidonoyl-glyceroland THC. The high in vivo potency of the novel short-chain saturatedMAFP derivatives (C8:0 and C12:0) underscores the complexity ofmanipulating the endogenous cannabinoidsystem.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Discovery of the endogenous cannabinoid anandamide provided crucial evidence for the existence of a naturally occurring cannabinoidsystem (Devane et al., 1992). It is well known that anandamideproduces most of the same pharmacological effects as $Delta$ ⁹-tetrahydrocannabinol ( $Delta$ ⁹-THC), including sedation, hypothermia, analgesia, and catalepsyin mice (Fride and Mechoulam, 1993; Smith et al., 1994), drugdiscrimination in rats and monkeys (Wiley et al., 1995, 1997;Jarbe et al., 1998), and overt behavior in dogs (Lichtman et al.,1998). Some differences have also been reported between anandamideand $Delta$ ⁹-THC. Clearly, anandamide has a much shorter duration of actionand is much less potent than $Delta$ ⁹-THC (Smith et al., 1994). These characteristics can be explainedin part by the rapid metabolism of anandamide and its brief presencein brain after the i.v. administration in rodents (Willoughbyet al., 1997).

As for other differences between anandamide and $Delta$ ⁹-THC, it was shown that in contrast to $Delta$ ⁹-THC, the antinociceptive effects of anandamide could not be alteredby modulators of cAMP and by $kappa$ -opioid receptor agonists and antagonists(Welch et al., 1995). Studies from our laboratory have failedto demonstrate antagonism of the effects of anandamide in micewith the CB1-selective antagonist SR 141716A [N-(piperidin-1-yl)-5-(4-chlorophenyl)-1(2,4-dichlorophenyl)-4-methyl-1H-pyrazole-3-carboxyamide],a compound that completely blocks the effects of $Delta$ ⁹-THC (Compton and Martin, 1997). Moreover, there have been tworeports of low doses of anandamide attenuating the effects of $Delta$ ⁹-THC (Fride et al., 1995; Welch et al., 1995). Closer examinationof the effects in the dog behavioral model revealed qualitativedifferences between anandamide and $Delta$ ⁹-THC (Lichtman et al., 1998). Although it is reasonable to speculatethat the pharmacological effects produced by the exogenous administrationof cannabinoids reflect the physiological role of endogenous cannabinoids,these pharmacological differences underscore the necessity ofcaution in making such an extrapolation. It may well be that theexogenous administration of cannabinoids elicits an exaggeratedresponse, such as the behavioral "high", which is atypical ofthe endogenoussystem.

Administration of the CB1 receptor antagonist SR 41716A provides another approach to manipulation of the endogenous system.It produces no behavioral effects in rodents at low to moderatedoses (Rinaldi-Carmona et al., 1994; Compton et al., 1996), whereashigher doses produced motor stimulation that could be due to eithera noncannabinoid effect of SR 141716A or blockade of endogenousanandamide (Compton et al., 1996). It also improved memory (Terranovaet al., 1996) and attenuated pain threshold at an extremely lowdose (Richardson et al., 1998), effects that could be due to manipulationof the endogenous anandamide or to inverse agonisteffects.

Manipulation of the synthesis and metabolism of anandamide represents still yet another approach to exploring the endogenouscannabinoid system. Metabolic inhibitors of anandamide includephenylmethylsulfonyl fluoride (PMSF; Deutsch and Chin, 1993; Childerset al., 1994), methylarachidonylfluorophosphonate (MAFP; De Petrocelliset al., 1997; Deutsch et al., 1997b), arachidonyl serotonin (Bisognoet al., 1998), and fatty acid sulfonyl fluorides (Deutsch et al.,1997a). PMSF has been shown to potentiate the effects of anandamideas well as produce some anandamide-like effects at high doses(Compton and Martin, 1997). Unfortunately, PMSF is a nonselectiveenzyme inhibitor, and no efforts were made to measure endogenousanandamide levels. The pharmacological profile of the other metabolicinhibitors has not been evaluatedthoroughly.

MAFP was initially designed and developed as the active-site directed inactivator of the calcium-sensitive and arachidonyl-selectivecytosolic phospholipase A₂ (Huang et al., 1966; Street et al.,1993). It has been shown to be a highly potent and selective inhibitorof fatty acid amidohydrolase activity (FAAH), the major enzymeresponsible for anandamide degradation (De Petrocellis et al.,1997; Deutsch et al., 1997b). Based on studies with related reagents(disopropylfluorophosphonate and ethoxyoleoyl fluorophosphonate)and site-directed mutagenesis studies, the mechanism of inhibitionwas found to involve the stable phosphorylation of an active-siteserine of FAAH (Hillard et al., 1995; Omeir et al., 1999; Patricelliet al., 1999).

MAFP bound irreversibly to the cannabinoid (CB1) receptor and prevented the subsequent binding of CP 55,940 (Deutsch et al.,1997b). In another study, it was found that MAFP acted as an irreversiblecannabinoid receptor antagonist in the electrically evoked isometriccontractions of the myenteric plexus-longitudinal muscle preparationof guinea pig small intestine (Fernando and Pertwee, 1997). Furthermore,in cardiac and invertebrate neural tissue, it enhanced anandamide-stimulatednitric oxide release (Bilfinger et al., 1998; Stefano et al.,1998). The goal of this study was to explore both in vivo andin vitro pharmacological actions of structural analogs of MAFP.Furthermore, efforts were made to determine whether the administrationof MAFP analogs could elevate anandamide and 2-arachidonoyl-glycerol(2-Ara-Gl) levels in brain and spinalcord.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

ICR male mice (Harlan Laboratories, Indianapolis, IN) weighing 24 to 26 g were used in all experiments. Mice were maintainedon a 14:10-h light/dark cycle with free access to food and water. $Delta$ ⁹-THC and SR 141716A were obtained from the National Instituteon Drug Abuse (Bethesda, MD). Anandamide and 2-Ara-Gl were synthesizedin our laboratory, and MAFP was obtained from Cayman Chemicals(Ann Arbor,MI).

Synthesis. The various methylfluorophosphonate analogs (Fig. 1) were prepared using a three-step synthetic sequence. Dimethyl phosphitewas alkylated by the appropriate iodo alkane derivative in thepresence of sodium hydride/N,N-dimethylformamide/tetrahydrofurateto give the corresponding dimethyl alkyl phosphonate (84-94% yield).Treatment of the phosphonate with sodium iodide in acetone furnishedthe corresponding methyl alkyl sodium phosphonate (70-75% yield),which was then allowed to react with (diethylamino)sulfur trifluorideto give the final methylfluorophosphonate derivative (60-80% yield).The experimental procedure for the synthesis of methyl octadecylfluorophosphonate (O-1623) is described below as a "general procedure"for all the analogs. The 1-iodo-(Z,Z)-11,14-eicosadiene and 1-iodo-(Z)-11-eicoseneused in the preparation of O-1625 and O-1626 were synthesizedfrom their respective alcohols (commercially available) usingstandard methodology by conversion to their mesylates (mesyl chloride/triethylamine/CH₂Cl₂)followed by treatment with NaI/CH₃CN/reflux (Ng et al., 1999).The iodo alkanes used in the synthesis of other analogs were allpurchased from Aldrich Chemical Co. ¹H NMR spectra were recorded on a JEOL Eclipse 300 spectrophotometerusing CDCl₃ as the solvent with tetramethylsilane as an internalstandard. Flash chromatography was carried out on EM Science (Gibbstown,NJ) silica gel 60. Elemental analyses were performed by AtlanticMicrolab, Inc. (Atlanta, GA).

View larger version (24K):
[in this window]
[in a new window]

Fig. 1. Structures of methylfluorophosphonate analogs.

Dimethyl Octadecyl Phosphonate. To a stirred suspension of sodium hydride (171 mg, 7.14 mmol) in DMF (9 ml) cooled to 0°C we added dropwise dimethyl phosphite(0.75 ml, 7.14 mmol). On addition, the mixture was warmed to roomtemperature and stirred for 1 h. A solution of 1-iodooctadecane(1.36 g, 3.59 mmol) in DMF/THF (1/1 8 ml) was then added dropwise,and the reaction mixture was stirred for 1 h. It was then quenchedwith water and extracted with ethyl acetate. The organic layerwas dried over MgSO₄ and evaporated under vacuum to yield dimethyloctadecyl phosphonate as a white solid (1.1 g, 84%): ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3 H, J = 6.6 Hz), 1.20 to 1.40 (m, 30H), 1.51 to1.79 (m, 4 H), 3.72 (d, 6 H, J = 10.7Hz).

Methyl Octadecyl Sodium Phosphonate. A stirred solution of methyl octadecyl phosphonate (650 mg, 1.8 mmol) and sodium iodide (540 mg, 3.6 mmol) in acetone (7 ml)was refluxed for 17 h. It was cooled to room temperature, andthe precipitated salt was filtered and washed with cold acetone.The salt was obtained as a white solid (486 mg, 73%) and usedwithout furtherpurification.

Methyl Octadecyl Fluorophosphonate (O-1623). To a stirred suspension of methyl octadecyl sodium phosphonate (200 mg, 0.54 mmol) in CH₂Cl₂ (9 ml) we added dropwise at roomtemperature (diethylamino)sulfur trifluoride (0.15 ml, 1.08 mmol).The reaction mixture was stirred for 1 h, quenched with water,and extracted with CH₂Cl₂. The organic layer was dried over MgSO₄,plugged through a pad of celite, and evaporated under reducedpressure. The residue was purified by flash chromatography (elutingwith hexane/EtOAc 2:1) to give methyl octadecyl fluorophosphonate(141 mg, 75%) as a yellowish solid: ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3 H, J = 6.6 Hz), 1.20 to 1.45 (m, 30H), 1.58 to 1.72 (m, 2 H), 1.82 to 1.96 (m, 2 H), 3.85 (dd, 3H, J = 0.8, 11.3 Hz). Analysis (C₁₉H₄₀O₂FP). Calculated: C 65.11,H 11.50. Found: C 65.07, H 11.54.

Methyl Octyl Fluorophosphonate (O-1887). Prepared in the same manner as methyl octadecyl fluorophosphonate in 84% yield: ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3 H, J = 6.6 Hz), 1.20 to 1.45 (m, 10H), 1.58 to 1.72 (m, 2 H), 1.82 to 1.96 (m, 2 H), 3.85 (dd, 3H, J = 0.8, 11.3 Hz). Analysis (C₉H₂₀O₂FP). Calculated: C 51.42,H 9.59. Found: C 51.19, H 9.57.

Methyl Dodecyl Fluorophosphonate (O-1778). Prepared in the same manner as methyl octadecyl fluorophosphonate in 84% yield: ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3 H, J = 6.6 Hz), 1.20 to 1.45 (m, 18H), 1.58 to 1.72 (m, 2 H), 1.82 to 1.96 (m, 2 H), 3.85 (dd, 3H, J = 0.8, 11.3 Hz). Analysis (C₁₃H₂₈O₂FP·0.4 H₂O). Calculated:C 57.08, H 10.61. Found: C 57.21, H 10.34.

Methyl Hexadecyl Fluorophosphonate (O-1705). Prepared in the same manner as methyl octadecyl fluorophosphonate in 60% yield: ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3 H, J = 6.6 Hz), 1.20 to 1.45 (m, 26H), 1.58 to 1.72 (m, 2 H), 1.82 to 1.96 (m, 2 H), 3.85 (dd, 3H, J = 0.8, 11.3 Hz). Analysis (C₁₇H₃₆O₂FP). Calculated: C 63.22,H 11.25. Found: C 63.42, H 11.18.

Methyl Eicosanyl Fluorophosphonate (O-1624). Prepared in the same manner as dimethyl octadecyl phosphonate in 80% yield: ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3 H, J = 6.6 Hz), 1.20 to 1.45 (m, 34H), 1.58 to 1.72 (m, 2 H), 1.82 to 1.96 (m, 2 H), 3.85 (dd, 3H, J = 0.8, 11.3 Hz). Analysis (C₂₁H₄₄O₂FP). Calculated: C 66.63,H 11.72. Found: C 66.73, H 11.83.

Methyl-(Z,Z)-11,14-eicosadienyl Fluorophosphonate (O-1625). Prepared in the same manner as methyl octadecyl fluorophosphonate in 60% yield: ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3H, J = 6.6 Hz), 1.20 to 1.45 (m, 20H), 1.58 to 1.72 (m, 2 H), 1.82 to 1.96 (m, 2 H), 2.04 (q, 4 H,J = 6.6 Hz), 2.76 (t, 2 H, J = 5.8 Hz), 3.85 (dd, 3 H, J = 0.8,11.3 Hz), 5.28 to 5.43 (m, 4 H). Analysis (C₂₁H₄₀O₂FP·0.5 H₂O).Calculated: C 65.76, H 10.77. Found: C 65.80, H 11.52.

Methyl-(Z)-11-eicosenyl Fluorophosphonate (O-1626). Prepared in the same manner as methyl octadecyl fluorophosphonate in 60%: ¹H NMR (CDCl₃) $delta$ 0.87 (t, 3 H, J = 6.6 Hz), 1.20 to 1.40 (m, 26H), 1.51 to 1.79 (m, 4 H), 2.00 (q, 4 H, J = 6.6 Hz), 3.85 (dd,3 H, J = 0.8, 12 Hz), 5.34 (t, 2 H, J = 5.9 Hz). Analysis (C₂₁H₄₂O₂FP·0.2CHCl₃). Calculated: C 63.59, H 10.62. Found: C 63.96, H 10.71.

Pharmacological Assays. Cannabinoids were dissolved in a 1:1:18 mixture of ethanol, emulphor, and saline for i.v. administration. Mice received theanalog by tail-vein injection and were evaluated for their abilityto produce hypomotility, hypothermia, and antinociception. Thesepharmacological measures were determined in the same mouse asdescribed earlier (Compton et al., 1993). To measure locomotoractivity, mice were placed into individual photocell activitychambers (11 × 6.5 inches) 5 min after injection. Spontaneousactivity was measured during the next 10-min period, and the numberof interruptions of 16 photocell beams per chamber was recorded.Antinociception was determined using the tail-flick reaction timeto a heat stimulus. Before vehicle or drug administration, thebaseline latency period (2-3 s) was determined. At 15 min afterthe injection, tail-flick latency was reassessed, and the differencesin control and test latencies were calculated. A 10-s maximumlatency was used. Antinociception was expressed as percentagemaximum possible effect (MPE) as described later. Regarding hypothermia,rectal temperature was determined before vehicle or drug administrationwith a telethermometer (Yellow Springs Instrument Co., YellowSprings, OH) and a thermistor probe (model YSI 400; Markson, Inc.,Hillsboro, OR) inserted at a depth of 2 mm. At 20 min after theinjection, rectal temperature was measured again, and the differencebetween preinjection and postinjection values was calculated.These pharmacological experiments were conducted between 8:00AM and 11:00PM.

For intrathecal (i.t.) administration, the methylfluorophosphonate derivatives were dissolved in 10% ethanol in dimethyl sulfoxide(DMSO). MAFP was prepared in DMSO alone. For i.t. administration,a 5-µl solution was injected into the spinal column between L5and L6 of unanesthetized mice with a 30-guage, 0.5-inch needle(Hylden and Wilcox, 1980

). The animals were tested for tail-flickresponse 5 min after theinjection.

The i.c.v. injections were performed in mice that were lightly anesthetized with ether. An incision was made in the scalpsuch that the bregma was exposed. Injections were performed usinga 26-guage needle with a sleeve of PE 20 tubing to control thedepth of the injection. An injection (5 µl) was made 2 mm rostraland 2 mm caudal to the bregma at a depth of 2 mm. The vehiclefor these injections consisted of 10% ethanol in DMSO. The animalswere tested 10 min after theinjection.

Receptor Binding. [³H]CP-55,940 (K_D = 690 nM) binding to P₂ membranes was conducted as described elsewhere (Compton et al., 1993), except wholebrain (rather than cortex only) was used. Displacement curveswere generated by incubating drugs with 1 nM [³H]CP-55,940. The assays were performed in triplicate, and theresults represent the combined data from three individual experiments.The K_i values were determined from displacement data using EBDA(Equilibrium Binding Data Analysis; BIOSOFT, Milltown,NJ).

FAAH Activity. The in vitro assay for FAAH activity was conducted using rat brain homogenate essentially as described earlier (Omeir et al.,1995). Frozen dissected brain (Pel-Freeze, Rogers, AR) was defrostedin 5 volumes of ice-cold Tris-EDTA, pH 7.6, and homogenized witha Polytron (Brinkmann Instruments, Westbury, NY). Aliquots ofthese brain homogenates were stored at $-$ 80°C. Incubations wereperformed in triplicate at 37°C in a water bath with shaking.Each incubation contained 10 µl of 50 mg/ml defatted BSA in H₂O(Sigma Chemical Co., St. Louis, MO), 10 µl of 20 mg/ml rat brainhomogenate protein, 30 µM anandamide (Cayman Chemical Co., AnnArbor, MI) plus 0.01 mCi of 120 mCi/mmol arachidonyl ethanolamide(ethanolamine-1,2-¹⁴C; New England Nuclear, Boston, MA), and 2 µl of various concentrationsof inhibitors dissolved in ethyl alcohol, in a final 200-µl incubationvolume of 0.1 M Tris-HCl (pH 9.0). The control tubes contained2 µl ethyl alcohol without inhibitor, and the blanks containedeverything except the rat brain. The reactions were terminatedby the addition of 2 volumes of chloroform/methanol (1:1). Theradioactivity in the aqueous phase was measured by liquid scintillationcounting. In a separate set of experiments, FAAH activity wasmeasured in ICR mouse spinal cord after i.t. treatment with O-1623and O-1624.

Anandamide and 2-AG Measurement in Tissues by Liquid Chromatography-Mass Spectrometry. At 10 min after i.t. treatment with either O-1623 or O-1624 (200 µg/mouse), ICR mouse spinal cords (one for each separatedetermination) were dissected and immediately frozen in liquidnitrogen, and so were the striata of ICR mice (two for each separatedetermination) after i.v. treatment with 30 mg/kg O-1624. Lipidextraction and prepurification was performed as described previouslyin the presence of 1 nmol of ²H₈-anandamide and 2 nmol of ²H₈-2-AG (Bisogno et al., 1999). Prepurified lipids were analyzedby HPLC-chemical ionization (APCI)-mass spectrometry. The massspectrometer was equipped with a Z-Spray APCI source operatingin the (+) APCI mode (source temperature 120°C, probe temperature110°C). N₂ was used as both drying and nebulizing gas (flow andprobe position were adjusted daily for optimum sensitivity). Thechromatograph was equipped with a Supelco Supelcosil LC-18 column(15 cm x 4.6 mm, 5 µm particle size). The mobile phase was MeOH/H₂O/aceticacid (85:15:0.2 by volume) at a flow rate of 1 ml/min. Both thecolumn and the samples were maintained at 25°C. Retention of peaksof a selected m/z value was used to identify anandamide and 2-AGin their protonated (M + 1) form. Quantification of the two compoundswas obtained by the isotope dilution method. After each injection,a 5 loop volume injection syringe purge waspreformed.

Data Analysis. For the production of hypomotility and hypothermia, the data were expressed as percentage of control activity and change intemperature (°C), respectively. Antinociception was calculatedas % MPE = [(test latency $-$ control latency)/(10 s $-$ control latency)]× 100. At least six animals were treated with each dose so dose-responserelationships could be determined for each analog. ED₅₀ valueswere determined from least-squares unweighted linear regressionanalysis of the log dose-response plots. Maximal effects for allcompounds combined on spontaneous activity, temperature, antinociception,and catalepsy were, respectively, 90% inhibition, $-$ 5°C, and 100%MPE. Thus, the ED₅₀ values indicate response levels of 45% inhibition, $-$ 2.5°C, and 50% MPE. Statistical analysis was carried out usingANOVA and Bonferroni/Dunn post hocanalysis.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Synthesis of Methylfluorophosphonate Analogs. Several analogs were prepared in which the alkyl moiety of the fluorophosphonate analog was varied as shown in Fig. 1. Initially,derivatives of MAFP were prepared by reducing the degree of unsaturationto either two double bonds to form methyl-(Z,Z)-11,14-eicosadienylfluorophosphonate (O-1625), one double bond to form methyl-(Z)-11-eicosenylfluorophosphonate (O-1626), or no unsaturation to form methyleicosanyl fluorophosphonate (O-1624). Then, three additional unsaturatedanalogs were prepared in which the alkyl group was reduced by2, 4, 8, and 12 carbon atoms to form methyl octadecyl fluorophosphonate(O-1623), methyl hexadecyl fluorophosphonate (O-1704), methyldodecyl fluorophosphonate (O-1778), and methyl octyl fluorophosphonate(O-1887),respectively.

Competition for [³H]CP 55,940 Binding. The ability of these analogs to compete with [³H]CP 55,940 binding is depicted in Fig. 2, top. MAFP was not analyzed becauseDeutsch et al. (1997b) previously reported that it displaced approximately90% of [³H]CP 55,940 binding with a IC₅₀ value of 20 nM. All of the analogs,with the exception of O-1624, effectively bound to the receptorat relatively low concentrations. However, none of these analogswas able to completely displace [³H]CP 55,940 binding, even at high concentrations. O-1625, theC20 analog with two double bonds, displaced approximately 70%of [³H]CP 55940 binding at 10 nM but was unable to displace a greaterquantity at concentrations up to 300 nM (Table 1). An estimatedK_i value of 2.9 ± 0.3 nM could be obtained. The C20 analog withone double bond, O-1626, was somewhat less effective in competingfor binding but presented a similar binding profile with 70% displacementat 1 µM. Again, analysis of the displacement curve yielded anestimated K_i value of 17 ± 2.4 nM. Complete saturation of theC20 analog resulted in O-1624, a compound with dramatically reducedreceptor affinity. The K_i value was determined to be 795 ± 72nM. Shortening the saturated chain resulted in a binding profilecomparable to that of O-1625 and O-1626 (Table 1). Maximal displacementby O-1623 (C18) was less than 70%, and a K_i value was estimatedto be 9.7 ± 1.5 nM. O-1705 (C16) produced only 58% displacementat the highest concentration, and a K_i value could not even beestimated. The binding profile of the C12 saturated analog O-1778was identical to that produced by O-1625 with regard to both maximaldisplacement (about 75%) and high receptor affinity (K_i = 2.54± 0.26 nM). However, shortening the chain to only eight carbonatoms (O-1887) completely eliminated CB1 receptor affinity.

View larger version (26K):
[in this window]
[in a new window]

Fig. 2. Displacement of [³H]CP 55940 binding to rat brain membranes. Top, competition of the methylfluorophosphonate analogs for [³H]CP 55940 binding. Bottom, influence of O-1624 (1 µM) and PMSF (50 µM) on the ability of anandamide to displace [³H]CP 55940 binding. The results in both experiments are presented as means ± S.E. of at least three separate displacements.

View this table:
[in this window]
[in a new window]

TABLE 1
Binding characteristics, FAAH inhibition, and pharmacological activity after i.v., i.t., and i.c.v. administration of the methylfluorophosphonate analogs

To compare the ability of PMSF and O-1624 to enhance anandamide binding to the cannabinoid receptor through FAAH inhibition,anandamide competition studies were conducted in the presenceof O-1624, PMSF, or the combination of both compounds. The resultsin Fig. 2 (bottom) demonstrate that O-1624 is approximately aseffective as PMSF in enhancing anandamide binding and that anandamidein the presence of the combination produced relatively the sameamount ofdisplacement.

FAAH Inhibition. All of the fluorophosphonates were highly potent inhibitors of FAAH in rat brain homogenates with IC₅₀ values in the nanomolarrange (Table 1). Interestingly, the least potent, O-1624, couldnot yield greater than 70 to 80% inhibition even at 500 nM. TheC12:0 compound, O-1778, was an extremely effective inhibitor.It yielded 50% inhibition of FAAH at 3 nM. Only two other compoundshave been reported to match this ability to inhibit FAAH undercomparable assay conditions: MAFP and laurylsulfonyl fluoride(De Petrocellis et al., 1997; Deutsch et al., 1997a,b; Di Marzoand Deutsch, 1998). Under the conditions of the assay with MAFP,it was estimated that approximately 10% of the cannabinoid receptorswould be occupied at concentrations of MAFP that inhibit 90% ofthe enzyme. For laurylsulfonyl fluoride, the ratio of the IC₅₀value for inhibition of FAAH versus competition for radioligandbinding at the receptor was approximately 7-fold, whereas othersulfonyl fluoride analogs showed higher selectivity for FAAH overthe CB1 receptor (Deutsch et al., 1997a).

Pharmacological Activity after i.v. Administration. The analogs were administered at doses as high as 30 mg/kg i.v. to mice and assessed for reductions in spontaneous activity,antinociceptive activity, and hypothermia. The results in Fig.3A and Table 1 show that the saturated C8:0 and C12:0 analogsO-1887 and O-1778 were highly potent and highly efficacious indepressing spontaneous activity. Its ED₅₀ value [95% confidencelimits (CL)] was 0.60 (0.5-0.7) and 0.60 (0.24-1.55) mg/kg, respectively.As for the other compounds, they depressed spontaneous activityat a dose of 30 mg/kg, but none produced maximal effects. Variableeffects were obtained with lower doses. Although the maximal effectsof O-1624 were only 54%, an ED₅₀ value (CL) of 26 (11-64) mg/kgcould be calculated (Table 1). Likewise, comparable ED₅₀ valuecould be calculated for O-1625 and O-1705. All of the compounds,with the exception of O-1624, produced a dose-related reductionin rectal temperature (Fig. 3B). Considering the maximal 6°C dropproduced by $Delta$ ⁹-THC, the only agonists that were as equally efficacious as $Delta$ ⁹-THC were O-1705 and O-1778 with ED₅₀ value of 10 and 3.2 mg/kg,respectively (Table 1). O-1625 exhibited similar potency, whereasO-1623 and O-1626 were considerably less potent and less efficacious.As for antinociception after i.v. administration, O-1887 and O-1778were the only analogs that produced dose-related antinociceptionwith maximal efficacy (Table 1). O-1705 was less potent but wascapable of producing approximately 70% MPE at 30 mg/kg. None ofthe other analogs was active even at doses as high as 30 mg/kg(Fig. 3C).

View larger version (18K):
[in this window]
[in a new window]

Fig. 3. The pharmacological effects of the methylfluorophosphonate analogs after i.v. administration in mice showing inhibition of spontaneous activity (A), depression of rectal temperature (B), and production of antinociception (C), respectively. The means ± S.E. represent at least six mice per group.

Given the fact that several of the analogs were capable of competing for [³H]CP 55,940 binding at very low concentrations yet produced modestpharmacological effects, a series of studies were carried outto determine whether they would either enhance or block the effectsof $Delta$ ⁹-THC. The results in Table 2 reveal that an i.v. dose of 10 mg/kgO-1623, O-1624, O-1625, and O-1626 produced some depression ofmotor activity, no antinociception, and very modest hypothermia.When these analogs were given before $Delta$ ⁹-THC, they failed to either potentiate or attenuate the actionsof the latter.

View this table:
[in this window]
[in a new window]

TABLE 2
Failure of methylfluorophosphonate derivatives to antagonize the pharmacological effects of $Delta$ ⁹-THC
Mice received a 10 mg/kg i.v. injection of the methylfluorphosphonate analog 10 min before a second i.v. injection of $Delta$ ⁹-THC (3 mg/kg), and the animals were evaluated for spontaneous activity (percentage of vehicle), tail-flick response (% MPE), and rectal temperature ( $Delta$ °C) at 5 to 15, 20, and 30 min after the last injection, respectively. The results are expressed as means ± S.E. for six mice per group.

The ability of O-1705 to produce hypoactivity, antinociception, and hypothermia suggested an interaction with the CB1 receptordespite its low receptor affinity. Therefore, SR 141716A was evaluatedto determine whether it would antagonize O-1705. O-1705 (30 mg/kg)administered i.v. produced a 30% reduction in spontaneous activity,69 ± 16% MPE, and a decrease of 4.7°C in body temperature. Pretreatmentwith SR 141716A (3 mg/kg i.v.) did not have a statistically significantinfluence on the effects of O-1705 on body temperature and spontaneousactivity but did produce a statistically significant antagonismof its antinociceptive effect (24 ± 17%).

Antinociceptive Activity after i.t. Administration. The activity of MAFP and the methylfluorophosphonate derivatives in the tail-flick procedure after i.t. administration ispresented in Fig. 4. MAFP produced a dose-responsive antinociceptiveeffect with an ED₅₀ value (CL) of 187 (156-224) µg/mouse. O-1625and O-1626 also produced a dose-responsive tail-flick responsewith ED₅₀ values of 111 (28-445) and 68 (17-268) µg/mouse. However,doses as high as 400 µg/mouse failed to produce maximal antinociception.O-1623 and O-1705 were only partially active, and O-1624 was withouteffect. On the other hand, O-1778 and O-1887 were fully efficaciousand highly potent with ED₅₀ values (CL) of 2.2 (1.5-3.3) and 7.7(2.9-21) µg/mouse, respectively. We also determined that a 10-minpretreatment with SR 141716A (10 or 30 mg/kg i.p.) failed to blockthe antinociception produced by MAFP (300 µg/mouse). MAFP produced92 ± 8% MPE in mice pretreated with vehicle and 79 ± 13 and 82± 13% MPE in mice receiving either 10 and 30 mg/kg SR 141716A(s.c.), respectively. An SR 141716A dose of 3 mg/kg completelyblocks an ED₈₄ dose of THC administered i.t.

View larger version (22K):
[in this window]
[in a new window]

Fig. 4. The antinociceptive effects of the methylfluorophosphonate analogs after either i.t. or i.c.v. administration to mice. The means ± S.E. represent at least six mice per group.

, 1623; $black-square$ , 1624; $open circle$ , 1625;

, 1626; $triangle$ , 1705; $black-triangle$ , MAPF; $oplus$ , 1778; $down-triangle$ , 1887.

To determine whether the inactive methylfluorophosphate analog O-1624 could potentiate the antinociceptive effects of anandamide,it was administered i.t. 10 min before an i.t. injection of anandamide.The results in Fig. 5, top, show that the ED₅₀ value (CL) of anandamide[23 (15-36) µg/mouse] was decreased to 9.0 (4.2-20), 3.6 (1.8-7.1),and 2.6 (1.6-4.1) as the dose of O-1624 was increased to 50, 100,and 200 µg/mouse, respectively. The two higher doses of O-1624produced statistically significant increases in that the CL valuesdo not overlap those of anandamide alone. The 200-µg dose of O-1624failed to alter the potency of either 2-ara-Gl or $Delta$ ⁹-THC as shown in the bottom two panels in Fig. 5. The ED₅₀ value(CL) values of 2-Ara-Gl after vehicle and O-1624 pretreatmentswere 29 (19-42) and 20 (14-29) µg/mouse, respectively. The ED₅₀value (CL) values of THC after vehicle and O-1624 pretreatmentswere 19 (13-28) and 18 (11-26) µg/mouse, respectively. Anothercompound that is capable of potentiating anandamide, PMSF, wasnot influenced by O-1624. An i.t. PMSF dose of 200 µg/mouse produced19 ± 7% and 26 ±8% MPE in the absence and presence of O-1624 (200µg/mouse), respectively (data not shown). Two other analogs werealso tested for their potential to augment the effects of anandamide.The ED₅₀ value (CL) of anandamide alone was decreased to 3.6 (1.6-8)µg/mouse when the mice were pretreated with a dose of 100 µg/mouseof O-1705 and to 8.8 (5.5-13.9) µg/mouse in mice pretreated withO-1623 (data not shown).

View larger version (12K):
[in this window]
[in a new window]

Fig. 5. The effect of O-1624 pretreatment on the antinociceptive effects of anandamide, 2-Ara-Gl, and $Delta$ ⁹-THC. Mice received a preinjection of either vehicle (

) or O-1624 (

, 50 µg; $black-square$ , 100 µg; $open circle$ , 200 µg) i.t. 10 min before a second i.t. injection of the cannabinoid and were tested 5 min after the last injection. The means ± S.E. represent at least six mice per group.

Antinociceptive Activity after i.c.v. Administration. The results in Fig. 4, bottom, show that O-1887, O-1778, and O-1626 were full antinociceptive agonists with respective ED₅₀value (CL) values of 11 (5-27), 20 (9-43), and 75 (28-204) µg/mouse(Table 1). O-1624 was without effect, and the other analogs producedless-than-maximaleffects.

Influence of O-1623 and O-1624 on Endocannabinoid Levels and FAAH Activity. The i.t. administration of these two compounds dramatically reduced FAAH activity in the spinal cord with little activitydetected with the more potent FAAH inhibitor O-1623. However,the anandamide levels were elevated only with the O-1624 analog,and neither compound altered 2-Ara-Gl levels. The i.v. administrationof O-1624 produced an elevation in both anandamide and 2-Ara-Glin the striatum, the only brain area studied (Table 3).

View this table:
[in this window]
[in a new window]

TABLE 3
Effect of O-1623 and O-1624 on FAAH activity and endogenous levels of anandamide and 2-Ara-Gl in spinal cord and striatum

Time Course Studies. The duration of action of these analogs is of considerable interest because of their potential for binding irreversibly toeither the receptor or to FAAH. The time course of O-1705, therelatively weak C16:0 analog, was evaluated after i.v. administration.The results in Fig. 6. demonstrate that this compound is stillexerting sedative, antinociceptive, and hypothermic effects at48 h after administration. The time course appears to consistof an early phase that partially recovers at 4 h, followed bya protracted second phase. Signs of toxicity were evident in theanimals at both 24 and 48 h, which could be due either to directeffects of the drug or to indirect effects arising from prolongedhypothermia along with compromised food and water intake. Thesesigns consisted primarily of loss of weight, lack of grooming,and lethargy.

View larger version (17K):
[in this window]
[in a new window]

Fig. 6. The time course of O-1705 effects after i.v. administration. Separate groups of mice were treated with either vehicle (

) or 10 ( $diamond$ ) or 30 ( $open circle$ ) mg/kg O-1705 and tested for spontaneous activity (top), tail-flick response (middle), and rectal temperature (bottom) at the indicated times. The means ± S.E. represent at least six mice per group.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

There are a large number of natural and synthetic inhibitors of endocannabinoid inactivation (see Di Marzo and Deutsch, 1998,for a recent review). Some of these agents interact with the CB1receptor, thereby suggesting some similarities between the recognitionsites on FAAH and the receptor. Previously, the structure-activityrelationship of a series of saturated fatty acid sulfonyl fluorideswas examined with regard to their ability to bind to the CB1 receptorand to inhibit FAAH (Deutsch et al., 1997a). The results obtainedherein with the saturated methylfluorophosphonates resemble someof the properties of the corresponding sulfonyl fluorides, butstriking differences exists. The C12:0 derivatives on both serieshad high affinity for the CB1 receptor, whereas there was a trendfor decreasing receptor affinity as the length of the alkyl groupincreased. However, the important difference between the two serieswas that the methylfluorophosphonates in the present study werenot capable of complete displacement of [³H]CP 55,940 binding, whereas the sulfonyl fluorides were. Forexample, the methylfluorophosphonate C16:0 at 10 µM displacedapproximately 50% of [³H]CP 55,940 binding, whereas the corresponding sulfonyl fluoridedisplaced more than 90%. Presently, it is unclear how some ofthese methylfluorophosphonate analogs are competing for receptorbinding at very low concentrations yet are incapable of maximaldisplacement. There are several possible explanations, the mostintriguing of which would be CP 55,940 binding to both sensitiveand nonsensitive methylfluorophosphonate sites. One cannot ruleout as-yet-unidentified factors that limit their accumulationat the binding site so that concentrations sufficient for completedisplacement cannot beachieved.

Regarding FAAH inhibition, the saturated sulfonyl fluoride C12:0 to C18:0 derivatives were all highly effective and of comparablepotency in blocking FAAH (Deutsch et al., 1997a). The C20:0 derivativeappeared to be least effective in blocking FAAH. Also, the C20:0methylfluorophosphonate was the lease active FAAH inhibitor inthe present study. In contrast, the C12:0 methylfluorophosphonatewas considerably more potent than all of the other analogs, whichwere of comparable potency regardless of alkyl length and degreeof saturation. On the other hand, the introduction of either oneor two unsaturated bonds to form either O-1626 or O-1625, respectively,enhanced receptor affinity with relatively little influence onFAAH inhibitory activity. It is therefore evident that the receptorprefers methylfluorophosphonates with short alkyl chains or longalkyl chains that are constrained, whereas the enzyme is considerablyless restrictive. Unfortunately, the influence of unsaturationof the alkyl group was not examined in the sulfonyl fluoride series(Deutsch et al., 1997a).

On i.v. administration, some of the methylfluorophosphonate analogs displayed potency and efficacy consistent with this bindingprofile. The finding that selected compounds were able to interactwith the CB1 receptor and act as either partial agonists or agonistsextends the cannabinoid structure-activity relationship. Mostfatty acid derivatives that have been evaluated for cannabinoideffects have been arachidonyl analogs. In this study, the C20analog with unsaturation at C11 and C14 (O-1625) exhibited thehighest receptor affinity and produced some effects on spontaneousactivity and hypothermia after i.v. administration. Saturatingthe C14 position (O-1626) slightly reduced affinity and pharmacologicalpotency. Obviously, the degree of unsaturation influences receptoraffinity for C20 analogs. The remaining compounds were saturatedwith varying chain length. Earlier, we had found that a fullysaturated anandamide derivative (C20:0) exhibited pharmacologicalpotency comparable to that of anandamide itself, but shorter chainderivatives were not explored (Adams et al., 1995). In contrast,the C20:0 saturated methylfluorophosphonate analog O-1624 exhibitedvery low affinity for the receptor and produced very little pharmacologicalactivity regardless of the route of administration. Shorteningthe chain by two carbons (O-1623) seemed to increase its abilityto bind to the receptor, but this analog was still quite weakpharmacologically. Reducing the chain length by two additionalcarbons led to O-1705, a compound that exhibited little affinityfor the receptor; yet, it was capable of producing dose-relatedeffects in all three assays after i.v. administration with potencycomparable to that of anandamide. It appears that this derivativeis not acting in a fashion identical to that of anandamide, becauseit was fully efficacious in reducing rectal temperature, whereasanandamide derivatives act as partial agonists in producing hypothermia.The high receptor affinity, in vivo potency, and efficacy resultingfrom further reduction of the alkyl chain to merely C12:0 (O-1778)were unexpected, particularly in light of our recent observationsthat extending and branching the alkyl chain in anandamide, tomimic a dimethylheptyl analog, enhanced CB1 receptor affinityand pharmacological potency (Ryan et al., 1997). This C12:0 derivativeprovides the clearest distinction between the structural requirementsof methylfluorophosphonates and anandamide-like derivatives forinteraction with the CB1 receptor. On the other hand, the findingthat the C8:0 analog failed to bind to the CB1 receptor, yet retainedhigh potency, demonstrates that this cannabinoid pharmacologicalprofile is not confined to this single receptor subtype. Furthermore,these observations raise the possibility that the other methylfluorophosphateanalogs are producing their effects through a combination of CB1and non-CB1 sites or solely non-CB1sites.

If the unsaturated analogs are indeed binding to the cannabinoid receptor to act as partial agonists, then they could actas antagonists of $Delta$ ⁹-THC. None of the analogs were able to attenuate the effects of $Delta$ ⁹-THC. However, it is important to point out that we have not beenable to reliably antagonize the in vivo effects of $Delta$ ⁹-THC unless we use antagonists with high receptoraffinity.

As mentioned earlier, the pharmacological effects of these compounds could be due to either CB1 receptor activation, FAAHinhibition, or to yet another mechanism. O-1623 and O-1624 producedonly minimal pharmacological effects after the i.v. administration,which is not surprising given their relatively weak receptor affinity,as discussed earlier. In particular, O-1624 elevated anandamidein both the spinal cord and the striatum (where 2-AG levels werealso elevated) under the same conditions necessary for this compoundto produce a small inhibitory effect on spontaneous activity butnot on the nociceptive response in the tail-flick test. Thesefindings suggest that the treatment of mice with this compoundis sufficient to raise endogenous anandamide levels in some tissuesbut not always to an extent necessary to exert a cannabimimeticaction. However, the observation that O-1623 was more potent thanO-1624 in inhibiting FAAH in the spinal cord after i.t. administrationbut paradoxically less potent in raising anandamide levels inthis tissue may suggest that the effects of these compounds onendogenous cannabinoid levels are not explained solely by theirinhibition of FAAH. On the other hand, O-1705 exerts activityat the receptor as well as FAAH inhibition similar to that ofO-1624 and O-1624, yet it is capable of producing pharmacologicalactivity after i.v. injection. This comparison suggests that O-1705is producing its effects through a non-CB1 receptor mechanism,as suggested earlier. This notion is further supported by thepotent C8:0 analog, which lacks affinity for CB1. The differencesbetween i.t. and i.v. administration of these analogs are alsoquite striking. The opposite pharmacological effects occurredwith O-1705, which was inactive when administered i.t., whereasO-1625 and O-1626 wereactive.

There is no question that O-1624 greatly potentiated the pharmacological effects of exogenously administered anandamide aswell as increased the ability of the latter to compete for CB1receptor binding, much in the same manner we demonstrated forPMSF (Compton and Martin, 1997). However, it appears that thisaction may have more relevance to metabolism of exogenous anandamidethan to endogenous cannabinoids. Although all of these MAFP analogsinhibit FAAH in brain homogenates, the degree to which they inhibitthe enzyme in vivo remains to be fully established. Their efficacydepends on their ability to be taken up into cells containingFAAH as well as their own metabolic stability. Furthermore, exogenousanandamide may be hydrolyzed by different FAAH-containing cellsthan the endogenoussubstance.

In conclusion, both saturated and unsaturated methylfluorophosphonate analogs inhibit FAAH. A short saturated alkyl chain(C12:0) derivative resulted in an highly potent agonist and aunique receptor probe. Failure of these analogs to completelydisplace [³H]CP 55,940 binding raises the possibility of subpopulations ofsites labeled by this ligand. The finding that the C8:0 analogwas highly potent in vivo yet failed to interact with the CB1receptor supports this notion. The inhibitory activity of theseanalogs at FAAH effectively retards the metabolism of exogenouslyadministered anandamide, but this action does not appear to contributeto their own pharmacological effects. It appears that these analogsare capable of producing at least some of their effects throughCB1 as well as non-CB1receptors.

	Footnotes

Accepted for publication May 2, 2000.

Received for publication February 11, 2000.

¹ This research was supported by National Institute on Drug Abuse Grant P01-DA09789. V.D.M. was the recipient of a Human Frontierin Science Program short-termfellowship.

Send reprint requests to: Dr. Billy R. Martin, Department of Pharmacology and Toxicology, Medical College of Virginia Campus, Virginia Commonwealth University, Box 980613, MCV Station, Richmond, VA 23298-0613. E-mail: Martinb{at}hsc.vcu.edu

	Abbreviations

THC, tetrahydrocannabinol; MPE, maximum possible effect; MAFP, methylarachidonylfluorophosphonate; PMSF, phenylmethylsulfonyl fluoride; FAAH, fatty acid amidohydrolase activity; 2-Ara-Gl, 2-arachidonoyl-glycerol; CL, confidence limits; i.t., intrathecal; DMSO, dimethyl sulfoxide.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

Adams IB, Ryan W, Singer M, Thomas BF, Compton DR, Razdan RK and Martin BR (1995) Evaluation of cannabinoid receptor binding and in vivo activities for anandamide analogs. J Pharmacol Exp Ther 273: 1172-1181[Abstract/Free Full Text].
Bilfinger TV, Salzet M, Fimiani C, Deutsch DG, Tramu G and Stefano GB (1998) Pharmacological evidence for anandamide amidase in human cardiac and vascular tissues. Int J Cardiol 64: S15-S22.
Bisogno T, Berrendero F, Ambrosino G, Cebeira M, Ramos JA, Fernandez-Ruiz JJ and Di Marzo V (1999) Brain regional distribution of endocannabinoids: Implications for their biosynthesis and biological function. Biochem Biophys Res Commun 256: 377-380[Medline].
Bisogno T, Melck D, De Petrocellis L, Bobrov MYu, Gretskaya NM, Bezuglov VV, Sitachitta N, Gerwick WH and Di Marzo V (1998) Arachidonoylserotonin and other novel inhibitors of fatty acid amide hydrolase. Biochem Biophys Res Commun 248: 515-522[Medline].
Childers SR, Sexton T and Roy MB (1994) Effects of anandamide on cannabinoid receptors in rat brain membranes. Biochem Pharmacol 47: 711-715[Medline].
Compton D, Aceto M, Lowe J and Martin B (1996) In vivo characterization of a specific cannabinoid receptor antagonist (SR141716A): Inhibition of $Delta$ ⁹-tetrahdrocannabinol-induced responses and apparent agonist activity. J Pharmacol Exp Ther 277: 586-594[Abstract/Free Full Text].
Compton DR and Martin BR (1997) The effect of the enzyme inhibitor phenylmethylsulfonyl fluoride on the pharmacological effect of anandamide in the mouse model of cannabimimetic activity. J Pharmacol Exp Ther 283: 1138-1143[Abstract/Free Full Text].
Compton DR, Rice KC, De Costa BR, Razdan RK, Melvin LS, Johnson MR and Martin BR (1993) Cannabinoid structure-activity relationships: Correlation of receptor binding and in vivo activities. J Pharmacol Exp Ther 265: 218-226[Abstract/Free Full Text].
De Petrocellis L, Melck D, Ueda N, Maurelli S, Kurahashi Y, Yamamoto S, Marino G and Di Marzo V (1997) Novel inhibitors of brain neuronal and basophilic anandamide amidohydrolase. Biochem Biophys Res Commun 231: 82-88[Medline].
Deutsch DG and Chin SA (1993) Enzymatic synthesis and degradation of anandamide, a cannabinoid receptor agonist. Biochem Pharmacol 46: 791-796[Medline].
Deutsch DG, Lin S, Hill WAG, Morse KL, Salehani D, Arreaza G, Omeir RL and Makriyannis A (1997a) Fatty acid sulfonyl fluorides inhibit anandamide metabolism and bind to the cannabinoid receptor. Biochem Pharmacol 53: 1-16[Medline].
Deutsch DG, Omeir R, Arreaza G, Salehani D, Prestwich GD, Huang Z and Howlett A (1997b) Methyl arachidonyl fluorophosphonate: A potent irreversible inhibitor of anandamide amidase. Biochem Pharmacol 53: 255-260[Medline].
Devane WA, Hanus L, Breuer A, Pertwee RG, Stevenson LA, Griffin G, Gibson D, Mandelbaum A, Etinger A and Mechoulam R (1992) Isolation and structure of a brain constituent that binds to the cannabinoid receptor. Science (Wash DC) 258: 1946-1949[Abstract/Free Full Text].
Di Marzo V and Deutsch DG (1998) Biochemistry of the endogenous ligands of cannabinoid receptors. Neurobiol Dis 5: 386-404[Medline].
Fernando SR and Pertwee RG (1997) Evidence that methyl arachidonyl fluorophosphate is an irreversible cannabinoid receptor antagonist. Br J Pharmacol 121: 1716-1720[Medline].
Fride E, Barg J, Levy R, Saya D, Heldman E, Mechoulam R and Vogel Z (1995) Low doses of anandamides inhibit pharmacological effects of $Delta$ ⁹-tetrahydrocannabinol. J Pharmacol Exp Ther 272: 699-707[Abstract/Free Full Text].
Fride E and Mechoulam R (1993) Pharmacological activity of the cannabinoid receptor agonist, anandamide, a brain constituent. Eur J Pharmacol 231: 313-314[Medline].
Hillard CJ, Wilkison D, Edgemond W and Campbell W (1995) Characterization of the kinetics and distribution of N-arachidonylethanolamine (anandamide) hydrolysis by rat brain. Biochim Biophys Acta 1257: 249-256[Medline].
Huang Z, Payette P, Abdullah K, Cromlish WA and Kennedy BP (1966) Functional identification of the active-site nucleophile of the human 85-kDa cytosolic phospholipase A2. Biochemistry 35: 3712-3721.
Hylden JL and Wilcox GL (1980) Intrathecal morphine in mice: A new technique. Eur J Pharmacol 67: 313-316[Medline].
Jarbe TU, Lamb RJ, Makriyannis A, Lin S and Goutopoulos A (1998) Delta-9-THC training dose as a determinant for (R)-methanandamide generalization in rats. Psychopharmacology (Berl) 140: 519-522[Medline].
Lichtman AH, Wiley JL, LaVecchia KL, Neviaser ST, Arthrur DB, Wilson DM and Martin BR (1998) Acute and chronic cannabinoid effects: Characterization of precipitated withdrawal in dogs. Eur J Pharmacol 357: 139-148[Medline].
Ng EW, Aung MM, Abood ME, Martin BR and Razdan RK (1999) Unique analogues of anandamide: Arachidonyl ethers and carbamates and norarachidonyl carbamates and ureas. J Med Chem 42: 1975-1981[Medline].
Omeir RL, Arreaza G and Deutsch DG (1999) Identification of two serine residues involved in catalysis by fatty acid amide hydrolase. Biochem Biophys Res Commun 264: 316-320[Medline].
Omeir RL, Chin S, Hong Y, Ahern DG and Deutsch DG (1995) Arachidonoyl ethanolamide-[1,2-C¹⁴] as a substrate for anandamide amidase. Life Sci 56: 1999-2005[Medline].
Patricelli MP, Lovato MA and Cravatt BF (1999) Chemical and mutagenic investigations of fatty acid amide hydrolase: Evidence for a family of serine hydrolases with distinct catalytic properties. Biochemistry 38: 9804-9812[Medline].
Richardson JD, Aanonsen L and Hargreaves KM (1998) Hypoactivity of the spinal cannabinoid system results in NMDA-dependent hyperalgesia. J Neurosci 18: 451-457[Abstract/Free Full Text].
Rinaldi-Carmona M, Barth F, Héaulme M, Shire D, Calandra B, Congy C, Martinez S, Maruani J, Néliat G, Caput D, Ferrara P, Soubrié P, Brelière JC and Le Fur G (1994) SR141716A, a potent and selective antagonist of the brain cannabinoid receptor. FEBS Lett 350: 240-244[Medline].
Ryan JW, Banner WK, Wiley JL, Martin BR and Razdan RK (1997) Potent anandamide analogs: The effect of changing the length and branching of the end pentyl chain. J Med Chem 40: 3617-3625[Medline].
Smith PB, Compton DR, Welch SP, Razdan RK, Mechoulam R and Martin BR (1994) The pharmacological activity of anandamide, a putative endogenous cannabinoid, in mice. J Pharmacol Exp Ther 270: 219-227[Abstract/Free Full Text].
Stefano GB, Rialas CM, Deutsch DG and Salzet M (1998) Anandamide amidase inhibition enhances anandamide-stimulated nitric oxide release in invertebrate neural tissues. Brain Res 793: 341-345[Medline].
Street IP, Lin HK, Laliberte F, Ghomashchi F, Wang Z, Perrier H, Tremblay NM, Huang Z, Weech PK and Gelb MH (1993) Slow- and tight-binding inhibitors of the 85-kDa human phospholipase A2. Biochemistry 32: 5935-5940[Medline].
Terranova JP, Storme JJ, Lafon N, Perio A, Rinaldi-Carmona M, Le Fur G and Soubrie P (1996) Improvement of memory in rodents by the selective CB1 cannabinoid receptor antagonist, SR 141716. Psychopharmacology 126: 165-172[Medline].
Welch SP, Dunlow LD, Patrick GS and Razdan RK (1995) Characterization of anandamide- and fluoroanandamide-induced antinociception and cross-tolerance to $Delta$ ⁹-THC following intrathecal administration to mice: blockade of $Delta$ ⁹-THC-induced antinociception. J Pharmacol Exp Ther 273: 1235-1244[Abstract/Free Full Text].
Wiley J, Balster R and Martin B (1995) Discriminative stimulus effects of anandamide in rats. Eur J Pharmacol 276: 49-54[Medline].
Wiley JL, Golden KM, Ryan WJ, Balster RL, Razdan RK and Martin BR (1997) Evaluation of cannabimimetic discriminative stimulus effects of anandamide and methylated fluoroanandamide in Rhesus monkeys. Pharmacol Biochem Behav 58: 1139-1143[Medline].
Willoughby KA, Moore SF, Martin BR and Ellis EF (1997) The biodisposition and metabolism of anandamide in mice. J Pharmacol Exp Ther 282: 243-247[Abstract/Free Full Text].

This article has been cited by other articles:

Y. Segall, G. B. Quistad, S. E. Sparks, D. K. Nomura, and J. E. Casida
Toxicological and Structural Features of Organophosphorus and Organosulfur Cannabinoid CB1 Receptor Ligands
Toxicol. Sci., November 1, 2003; 76(1): 131 - 137.
[Abstract] [Full Text] [PDF]

S. T. Glaser, N. A. Abumrad, F. Fatade, M. Kaczocha, K. M. Studholme, and D. G. Deutsch
Evidence against the presence of an anandamide transporter
PNAS, April 1, 2003; 100(7): 4269 - 4274.
[Abstract] [Full Text] [PDF]

D. G. Deutsch, S. T. Glaser, J. M. Howell, J. S. Kunz, R. A. Puffenbarger, C. J. Hillard, and N. Abumrad
The Cellular Uptake of Anandamide Is Coupled to Its Breakdown by Fatty-acid Amide Hydrolase
J. Biol. Chem., March 2, 2001; 276(10): 6967 - 6973.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit a response

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Similar articles in this journal

Similar articles in PubMed

				S. T. Glaser, N. A. Abumrad, F. Fatade, M. Kaczocha, K. M. Studholme, and D. G. Deutsch Evidence against the presence of an anandamide transporter PNAS, April 1, 2003; 100(7): 4269 - 4274. [Abstract] [Full Text] [PDF]

				D. G. Deutsch, S. T. Glaser, J. M. Howell, J. S. Kunz, R. A. Puffenbarger, C. J. Hillard, and N. Abumrad The Cellular Uptake of Anandamide Is Coupled to Its Breakdown by Fatty-acid Amide Hydrolase J. Biol. Chem., March 2, 2001; 276(10): 6967 - 6973. [Abstract] [Full Text] [PDF]

Cannabinoid Properties of Methylfluorophosphonate Analogs1

Cannabinoid Properties of Methylfluorophosphonate Analogs¹