U937 cells deprived of endogenous annexin 1 demonstrate an increased PLA2 activity

Abstract

Annexin 1 (An 1), a phospholipid and calcium binding protein, is strongly expressed in differentiated U 937 cells. In attempting to correlate the expression of An 1 with phospholipase A₂ (PLA₂) activity, U 937 cells were stably transfected both with a Sense and Antisense cDNA for An 1. PLA₂ activity was measured by Flow cytometry analysis utilizing the bis‐Bodipy‐C₁₁‐PC fluorescent probe. U 937 cells stably transfected with the sense or antisense vectors were differentiated for 24 h with phorbol 12‐myristate 13‐acetate (PMA, 6 ng ml⁻¹). Both in undifferentiated and differentiated cells, the Antisense clone (36.4 AS) showed consistently higher PLA₂ activity than the control Sense clone (15 S). Since the fluorescent probe measures the total PLA₂ activity, we used two different stimuli, PMA: (100 ng ml⁻¹) or lipopolysaccharide (LPS, 10 ng ml⁻¹), and two different inhibitors, to discriminate the PLA₂ involved (namely arachidonyl trifluoromethyl ketone or AACOCF3, which is specific for the cytosolic PLA₂, and SB 203347 specific for the secretory PLA₂). In the Antisense clone the inhibitory effect of AACOCF was stronger [68%, P2 activity is correlated with its phosphorylation, Western and shift blot analysis were performed. They did not show any significative difference between the phosphorylated and non phosphorylated form of the enzyme in both the differentiated or not, Sense and Antisense clones. Furthermore the tyrosine phosphorylation analysis of An 1 showed that less than 10% of An 1 was phosphorylated irrespective of PMA presence or absence. From the pattern of inhibition observed, we propose that the endogenous unphosphorylated form of An 1 may act intracellularly to block the activity of a cytosolic PLA₂. British Journal of Pharmacology (1998) 124, 1675–1683; doi:10.1038/sj.bjp.0701991