Inositol triphosphate Neutrophils at a concentration selleck kinase inhibitor of 5 106. ml 1 in Ca2 replete HBSS were preincubated for 10 min at 37 C in the presence or absence of GF10903 , followed by the addition of PAF or FMLP in a final volume of 2 ml, after which the reactions were terminated and the IP3 e tracted by the addition of 0. 4 ml of 20% per chloric acid at 10 and 20 sec after addition of the chem oattractant, and the tubes transferred to an ice bath. These incubation times coincide with the early peak IP3 responses of PAF activated neutrophils, as well as the subsequent decline towards basal levels which are reached at around 60 sec, determined in a series of preliminary e periments. In an additional series of e periments, the effects of the PKC activator, phorbol 12 myristate 13 acetate on the IP3 responses of PAF activated cells in the absence and presence of GF10903 were investigated.

Following 20 min incubation on ice, the tubes were cen trifuged at 2000 g for 15 min and the supernatants removed and brought to pH 7. 5 with 5N KOH, followed by centrifugation at 2000 g for 15 min to remove precip itated perchloric acid. The supernatants were assayed using the inositol 1,4,5 triphosphate radioreceptor assay procedure, which is a competitive ligand binding assay, and the results e pressed as pmol IP3 107 cells. Measurement of LTB4 A competitive binding enzyme immunoassay procedure was used to measure LTB4 in the supernatants of neu trophils activated with PAF in the absence or presence of GF10903 .

Neutrophils in HBSS were preincubated for 10 min at 37 C with the test agent after which PAF was added to the cells and the reactions stopped after 3 min incubation at 37 C by the addition of an equal volume of ice cold HBSS to the tubes which were then held in an ice bath prior to pelleting the cells by centrifugation. The cell free supernatants were then GSK-3 assayed for LTB4 using the enzyme immunoassay procedure. Supernatants from cells activated with PAF were diluted 1 4 prior to assay. These results are e pressed as picograms 107 cells. Statistical Analysis The results of each series of e periments are e pressed as the mean value standard error of the mean, with the e ception of the fura 2 AM e periments for which the traces are also presented. Levels of statistical significance were calculated using paired Stu dents t test when comparing two groups, or by analysis of variance with subsequent Tukey Kramer multi ple comparisons test for multiple groups. A P value 0. 05 was considered significant. GF10903 fluorescenceofresponsesstaurosporinenM activatedofneu Ca2 concentrations that declined towards resting levels at significantly slower rates than those observed for control systems.