AEA-induced apoptosis of CxCa cell lines. (A) The viability of healthy donor PBLs (black square), CC299 (black triangle), Caski (white circle) and Hela cells (black circle) was assessed in a MTT assay after 5 days of AEA exposure. AEA was added daily in culture medium because of its high instability. Vehicle consisted in ethanol and never exceeded 1% of the final culture medium volume. Results are expressed as mean ± SD of triplicates. (B) Flow cytometry analysis of DNA fragmentation of CC299 cell line exposed to 30 μM AEA for 0, 15, 24, 48 and 72 h. Similar DNA content patterns were obtained with Caski and HeLa cells (percentages of cells in sub-G0/G1 reported in C for each cell line). (C) Kinetics analysis of the sub-G0/G1 cell fraction (fragmented DNA) in CxCa cells treated with 30 μM AEA (black circle) or vehicle (white circle). Results are expressed as mean ± SD of duplicates. (D) Western blot analysis of caspase-7 activation in CC299 cells. Cleaved form of caspase-7 (20 kDa) was observed 48 h after addition of 30 μM AEA.

CB1, CB2 and VR1 are expressed by CxCa cell lines. Expression of cannabinoid receptors was assessed by RT-PCR (A) and Western blot analysis (B). Expected protein size was 84 kDa for VR1, 52 kDa for CB1 and 38 kDa for CB2.

VR1 is involved in AEA-induced death of cervical cancer cells, whereas CB1 and CB2 are protective. Viability of CC299, Caski and HeLa cell lines was assessed by MTT assay after 3 days (black histogram) or 5 days (gray histogram) of AEA exposure. Antagonists to CB1 (SR1, 0.2 μM), CB2 (SR2, 0.2 μM) and VR1 (capsazepine, CZ, 0.5 μM) were added 15 min before addition of 30 μM AEA. Results are expressed as mean ± SD of triplicates.

Expression of receptors to AEA in cervix malignancies. RT-PCR analysis using specific primers for VR1, CB1 and CB2 was performed on stage Ib–II CxCa biopsies.