IL-1beta induces alkaline phosphatase in human phagocytes

Background. Alkaline phosphatase (ALPase) is found in blood plasma or serum and leukocytes and regulates intercellular processes, maintaining phosphoryl metabolites in a steady state, as well as synthesizing and hydrolyzing phosphate esters on membranes. ALPase supervises the active transport of inorganic phosphates, fats, proteins, carbohydrates and the sodium/potassium pump mechanisms. The formed elements of blood such as polymorphonuclear (PMNs) leucocytes, macrophages (MP) and some lymphocytes are high in ALPase concentrations. Methods. In this study we have tested whether the interleukin-1 receptor antagonist (IL-1ra) could influence ALPase generation in IL-1 beta or lipopolysaccharide (LPS)-stimulated neutrophils and MP. Human neutrophils were isolated from heparin-anticoagulated blood drawn from healthy individuals by centrifugation in a two-step gradient, Ficoll-Hypaque. ALPase activity was assessed spectrophotometrically in test tubes containing isolated neutrophils and adherence PBMCs treated with LPS, IL-1 beta and IL-1ra, alone or in combination. Results. IL-1 beta or LPS enhanced ALPase in both PMNs and MP, whereas IL-1ra could not inhibit ALPase activity. We performed time course experiments at 0 min, 5 min, I h, 24 h, and 43 h (LPS 20 mu g/mL, IL-1 beta 10 ng/mL). No significant increase in ALPase activity was seen until 1 h; however, there was a rapid rise over the next few hours. In another set of experiments using IL-1ra (500 ng/mL), there was no difference between treated cells and control cells. The combination of IL-1 beta plus IL-1ra did not reduce the ability of ILAP to induce ALPase activity. Conclusions. These data suggest that IL-1 beta stimulates ALPase through other mechanisms than the release of arachidonic acid products, which are inhibited by IL-1ra. (C) 2007 IMSS. Published by Elsevier Inc.