Abstract
We have shown previously that guinea pig alveolar macrophages (AM) synthesize a secretory phospholipase A2 (PLA2) during in vitro incubation. Here, we report the molecular cloning of this enzyme and show that it has structural features closely related to all known mammalian type-II PLA2. The mRNA and PLA2 activity were undetectable in freshly collected AM, but their levels increased dramatically to reach maximal values after 16 h of culture. Thereafter, the PLA2 activity remained constant with a parallel secretion in the medium, in contrast to mRNA level which returned to near basal values after 32 h. Incubation of AM for 16 h with the inflammatory secretagogue peptide f-Met-Leu-Phe (fMLP) markedly reduced the PLA2 activity and mRNA levels. This inhibition was prevented by preexposure of AM to pertussis toxin, an inhibitor of G-protein. In contrast, when AM were first cultured for 16 h and then incubated with fMLP, no significant change was observed in their PLA2 activity. In conditions where the type-II PLA2 was completely abrogated by fMLP, the latter did not alter the lipopolysaccharide-induced accumulation of tumor necrosis factor alpha mRNA or the release of arachidonic acid induced by the subsequent addition of the calcium ionophore A23187. These studies show that the inflammatory peptide fMLP down-regulates the expression of the type-II PLA2 by AM through a process mediated by G-protein. A possible negative control of the type-II PLA2 expression during AM activation is suggested.
Highlights
From the tUnite de Pharmacologic Cellulaire, Unite Associee Pasteur, INSERM U285, the ~Unite de Genetique et de Biochimie du Deoeloppement, Unite Associee Pasteur/CNRS URA 361, and Institut Pasteur, 25 rue Dr Roux, 75015 Paris, France
Th e PLAz activi ty produced by t ra ns fecte d COS cells ha d cha racte ristics si milar to t hose of guinea pig alveolar macrophages (AM) [6] and oth er mammali a n ty pe-II phospholipase A:a (PLA) z [3,4,5]
Expression of the Typ e-Il PLA2 in AM, peritonea l macrophages (PM), and peripheral blood monocyt es (PBM)-The ty pe-II PLAz acti vity an d mRNA wer e undet ectabl e wh en freshly collect ed AM were allowed to a dhere for 1 h in the pr esenc e of 3% fetal calf serum (FCS)
Summary
From the tUnite de Pharmacologic Cellulaire, Unite Associee Pasteur, INSERM U285, the ~Unite de Genetique et de Biochimie du Deoeloppement, Unite Associee Pasteur/CNRS URA 361, and Institut Pasteur, 25 rue Dr Roux, 75015 Paris, France. In conditions where the type-II PLA:a was completely abrogated by fMLP, the latter did not alter the lipopolysaccharide-induced accumulation of tumor necrosis factor a mRNA or the release of arachidonic acid induced by the subsequent addition of the calcium ionophore A23187 These studies show that the inflammatory peptide fMLP down-regulates the expression of the type-II PLA:a by AM through a process mediated by G-protein. Phospholipases ~ (pLAz, phosphatide 2-acylhydrolase, EC 3.1.1.4) are widely distributed enzymes [1] abundant in pancreatic juice and in the venoms of snakes and bees, in which they serve digestive functions They are present in trace amounts in mammalian cells and are involved in the turnover and remodeling of membrane phospholipids.
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