Development of the first potential covalent inhibitors of anandamide cellular uptake.

On the basis of the chemical structures of two previously developed metabolically stable and relatively potent inhibitors of anandamide uptake, OMDM-1,2, two series of potential covalent inhibitors of anandamide cellular reuptake, which might be used for the molecular characterization of the protein(s) involved in the membrane transport of endocannabinoids, have been designed and synthesized. Most of the compounds inhibited uptake to a varied extent and in a generally enantio-sensitive manner when co-incubated with [(14)C]anandamide, but only three of them, the photoactivatable 1a (OMDM-37), 1b (OMDM-39), and 8(Lo395), also produced a significant inhibition of uptake following the preincubation only of the cells, and this effect was significantly enhanced following UV exposure only in the case of 8. None of the new compounds inhibited [(14)C]anandamide hydrolysis with IC(50) < 50 microM, except for 1b.

High affinity electrophilic and photoactivatable covalent endocannabinoid probes for the CB1 receptor.

We have designed and synthesized the first two high affinity covalent anandamide probes for the CB1 receptor by introducing either an electrophilic isothiocyanato or a photoactivatable azido group at the terminal carbon of the arachidonic acid moiety. The headgroup of these anandamide analogues was optimized by using a cyclopropylamide substituent to impart optimal CB1 affinity. Both 20-isothiocyanato-eicosa-5,8,11,14-tetraenoic acid cyclopropylamide (1, AM3677) and 20-azido-eicosa-5,8,11,14-tetraenoic acid cyclopropylamide (2, AM3661) exhibited high selectivities for the CB1 receptor with K(i) values of 1.3 and 0.9 nM, respectively. Using suitable experimental conditions, both ligands were shown to covalently label the CB1 receptor with high efficiency. These two covalent probes for the endocannabinoid CB1 binding site open the door for exploring the ligand binding motifs involved in the activation of the CB1 receptor by its endogenous ligand, anandamide.

Gas chromatographic analysis of reactive carbonyl compounds formed from lipids upon UV-irradiation.

Peroxidation of lipids produces carbonyl compounds; some of these, e.g., malonaldehyde and 4-hydroxynonenal, are genotoxic because of their reactivity with biological nucleophiles. Analysis of the reactive carbonyl compounds is often difficult. The methylhydrazine method developed for malonaldehyde analysis was applied to simultaneously measure the products formed from linoleic acid, linolenic acid, arachidonic acid, and squalene upon ultraviolet-irradiation (UV-irradiation). The photoreaction products, saturated monocarbonyl, alpha,beta-unsaturated carbonyls, and beta-dicarbonyls, were derivatized with methylhydrazine to give hydrazones, pyrazolines, and pyrazoles, respectively. The derivatives were analyzed by gas chromatography and gas chromatography-mass spectrometry. Lipid peroxidation products identified included formaldehyde, acetaldehyde, acrolein, malonaldehyde, n-hexanal, and 4-hydroxy-2-nonenal. Malonaldehyde levels formed upon 4 hr of irradiation were 0.06 micrograms/mg from squalene, 2.4 micrograms/mg from linolenic acid, and 5.7 micrograms/mg from arachidonic acid. Significant levels of acrolein (2.5 micrograms/mg) and 4-hydroxy-2-nonenal (0.17 micrograms/mg) were also produced from arachidonic acid upon 4 hr irradiation.

UVB irradiation and distribution of arachidonic acid (20:4) and stearic acid (18:0) in human keratinocytes.

Human keratinocytes (NCTC 2544) in culture were labeled with either 14C-arachidonic acid or 14C-stearic acid and then exposed to UVB irradiation (9 or 90 mJ/cm2). Exposure of the keratinocytes to UVB irradiation resulted in considerable rearrangement of the membrane fatty acids. Following UVB irradiation the percentage amounts of 14C-arachidonic acid and 14C-stearic acid were significantly decreased in phospholipids, in phosphatidylethanolamine and in phosphatidylcholine. The liberation of stearic acid from phospholipids was accompanied by accumulation of radiolabel into the culture medium, but in 14C-arachidonic acid-labeled cells the amount of radiolabel in the culture medium was not changed following UVB irradiation despite liberation of arachidonic acid from phospholipids. It seems evident that, following UVB irradiation, the rate of reincorporation of liberated 14C-arachidonic acid, a polyunsaturated fatty acid, is higher and thus different from that of a saturated fatty acid, 14C-stearic acid. The present study suggests that exposure of keratinocytes to UVB irradiation is followed by liberation of both saturated and unsaturated fatty acids and also considerable reacylation of the unsaturated fatty acids.

Light exposure stimulates arachidonic acid metabolism in intact rat retina and isolated rod outer segments.

This paper presents evidence that short-term exposure to light increases synthesis of hydroxyeicosatetraenoic acid (HETE) and prostaglandin D2 (PGD2) and stimulates the uptake and metabolism of 20:4 in phospholipids and triacylglycerols in rat retina. There was a time-dependent increase in incorporation of 1-14C-20:4 into glycerolipids in both dark-adapted and light-exposed groups. Exposure to light for 15 or 30 min enhanced the acylation of 20:4 into phosphatidylcholine, phosphatidylinositol, phosphatidylethanolamine and triacylglycerols. In the light-exposed groups there was a large increase in the conversion of 20:4 to leukotriene B4, two diHETEs, 5-HETE, 15-HETE, and PGD2. The stimulation of HETE synthesis by light could be due to early stages of light-induced lipid peroxidation in visual cells. To examine this, we studied peroxidation of 20:4 in isolated rod outer segments (ROS). There was more oxidation of 20:4 in light-exposed ROS, as compared to ROS incubated in the dark. Vitamin E and nordihydroguaiaretic acid inhibited the light-induced formation of some of these products. The data indicate that photo-oxidation of 20:4 in ROS is accompanied by enzymatic oxygenation that is stimulated by light. Increased production of HETEs an PGD2 may be a consequence of the light-induced stimulation of the metabolism of 20:4 in membrane phospholipids in the retina.

Membrane responses of B-16 melanoma cells to single exposure to ultraviolet light.

Electron spin resonance spectroscopy using the spin probe (5-, 12- and 16-deoxylstearic acid) was employed to analyze the changes in membrane fluidity in B-16 melanoma cells following UV-B exposure. The UV exposure resulted in the immediate accumulation of lipid peroxide, being accompanied by a change in membrane fluidity. The 12-DSA is the most sensitive to the changes in membrane organization caused by UV light. Na+,K+-ATPase activity was regulated by a change in membrane fluidity. Following UV exposure, the release of the prelabeled arachidonic acid from the cells was observed immediately. Ca2+-dependent calmodulin-dependent phospholipase A2-like activity was involved in the UV-stimulated arachidonic acid release from phospholipid.

Influence of whole-body gamma irradiation upon arachidonic acid metabolism in rat platelets.

The effects of whole-body gamma irradiation (8.4 Gy) were studied on arachidonic acid (AA) metabolism in rats' blood platelets, from day D + 1 to day D + 10 after irradiation. AA conversion into thromboxane B2 (TxB2) increased at D + 1 and then gradually decreased to very low values from D + 7 to D + 10. This decrease in the conversion of exogenous AA into TxB2 was due to a lower AA incorporation into platelets and not to a decrease of cyclooxygenase and thromboxane-synthetase activities. AA incorporation into membrane phospholipids of blood platelets was much more decreased than AA incorporation into whole platelets; moreover, the lipid composition of the platelet membranes was markedly modified after irradiation, which must have resulted in structural and functional changes in these membranes; from these effects of whole-body gamma irradiation on platelets, the latter's membranes appeared as a major site of in vivo radiation damage in these cells.

Comparison of the radiosensitivity of unsaturated fatty acids, structured as micelles or liposomes, under different experimental conditions.

A comparison has been made between the peroxidation rate as a result of ionizing radiation in liposomes prepared from phospholipids which were extracted from biological membranes, in single component micelles and in micelles of mixed composition. The ease of fatty acid oxidation in the different preparations was studied at a variety of pH values. The damage has been quantified spectrophotometrically in terms of diene conjugation (233 nm) and as the disappearance of fatty acids by gas chromatography. The ease of fatty acid oxidation was in the following order for the liposomal and mixed micelle preparations: 22:6 greater than 20:4 greater than 18:2. For single component micelles the order was reversed: 18:2 greater than 18:3 greater than 20:4 greater than 22:6. The micellar lipid preparations were pH-dependent in their response to radiation, which was demonstrated by a dip in the pH-response curve. Peroxidation of especially 22:6 was promoted when present in mixed micelles with 18:2.

[Free radical oxidation of biological membrane lipids. VII. Effect of ultraviolet radiation on free radical oxidation of lipids complexed with protein and in biomembranes]. / Svobodnoradikal'noe okislenie lipidov biologicheskikh membran. VII. Deistvie ul'trafioletovogo izlucheniia na svobodnoradilak'noe okislenie lipidov v komplekse s belkom i v biomembranakh

Promoting effect of protein component on the development of free radical oxidation in the systems ethylarahidonate--bovine serum albumin and mitochondria suspension under UV irradiation has been shown. Connection between the processes of peroxide formation and the change of the functional activity of organells has been followed.