Stimulation of p38 Phosphorylation and Activity by Arachidonic Acid in HeLa Cells, HL60 Promyelocytic Leukemic Cells, and Human Neutrophils

Although it is well appreciated that arachidonic acid, a second messenger molecule that is released by ligand-stimulated phospholipase A2, stimulates a wide range of cell types, the mechanisms that mediate the actions of arachidonic acid are still poorly understood. We now report that arachidonic acid stimulated the appearance of dual-phosphorylated (active) p38 mitogen-activated protein kinase as detected by Western blotting in HeLa cells, HL60 cells, human neutrophils, and human umbilical vein endothelial cells but not Jurkat cells. An increase in p38 kinase activity caused by arachidonic acid was also observed. Further studies with neutrophils show that the stimulation of p38 dual phosphorylation by arachidonic acid was transient, peaking at 5 min, and was concentration-dependent. The effect of arachidonic acid was not affected by either nordihydroguaiaretic acid, an inhibitor of the 5-, 12-, and 15-lipoxygenases or by indomethacin, an inhibitor of cyclooxygenase. Arachidonic acid also stimulated the phosphorylation and/or activity of the extracellular signal-regulated protein kinase and of c-jun N-terminal kinase in a cell-type-specific manner. An examination of the mechanisms through which arachidonic acid stimulated the phosphorylation/activity of p38 and extracellular signal-regulated protein kinase in neutrophils revealed an involvement of protein kinase C. Thus, arachidonic acid stimulated the translocation of protein kinase C α, βI, and βII to a particulate fraction, and the effects of arachidonic acid on mitogen-activated protein kinase phosphorylation/activity were partially inhibited by GF109203X, an inhibitor of protein kinase C. This study is the first to demonstrate that a polyunsaturated fatty acid causes the dual phosphorylation and activation of p38.

Arachidonic acid (20:46) 1 is a second messenger that is released by the action of phospholipase A 2 in activated cells (1). In in vitro assays, 20:46 and other polyunsaturated fatty acids have been demonstrated to stimulate the activity of protein kinase C (PKC) (2, 3). When added exogenously, 20:46 is biologically active in a wide spectrum of cells. For example, 20:46 has been reported to inhibit gap junctional permeability between adherent cells (4); stimulate superoxide production and degranulation and increase the expression of CD11b/CD18 in human neutrophils (5)(6)(7), prime macrophages, and monocytes for enhanced respiratory burst (8); stimulate insulin secretion from isolated islets of Langerhans (9); modulate the permeability of K ϩ , Na ϩ , and H ϩ channels in a variety of cell types (10 -12); stimulate gene transcription (13); and cause differentiation and death (14). However, the molecular mechanisms through which the actions of 20:46 are mediated are poorly understood.
We have previously demonstrated that 20:46 and other polyunsaturated fatty acids stimulate the activity of the extracellular signal-regulated protein kinase (ERK) in WB rat liver epithelial cells (15), suggesting that ERK may mediate some of the biological actions of polyunsaturated fatty acids. Others have reported that arachidonic acid and its metabolites stimulate ERK activity in smooth muscle cells (16). ERK and the closely related p38 and jun N-terminal kinase (JNK) are members of the mitogen-activated protein (MAP) kinase family of kinases (17). These kinases are activated when cells are exposed to growth factors, cytokines, and/or various forms of stress (17,18). Activation of ERK, JNK, and p38 MAP kinases are achieved through the dual phosphorylation of threonine and tyrosine residues in the TXY motif by upstream MAP kinase kinases. MAP kinases have been proposed to regulate a diverse range of biological functions, including cytokine production and cell growth, differentiation, and death (17,18). Although 20:46 has recently been reported to stimulate the activity of JNK in proximal tubular epithelial cells and in stromal cells (19,20), we are not aware of any studies that have investigated whether 20:46 affects the activity of p38. We now report the novel finding that 20:46 stimulated the dual phosphorylation of p38 in HeLa cells, HL60 cells, human umbilical vein endothelial cells, and human neutrophils but not in Jurkat T cells. Further characterization in neutrophils demonstrated that 20:46 also stimulated the phosphorylation/activity of ERK but not of JNK, although the activity of JNK was weakly stimulated by 20:46 in Jurkat cells. 20:46 also stimulated the translocation of a number of PKC isozymes to a particulate fraction in neutrophils. The effect of 20:46 on p38 and ERK dual phosphorylation/activity was partially blocked by GF109203X, a specific inhibitor of PKC. These data demonstrate that the ability of 20:46 to stimulate the activity of p38 and JNK is cell typedependent and suggest that p38, ERK, JNK, and PKC are potential mediators of the biological actions of 20:46.

Materials
Fatty acids, 20:46, formyl-methionyl-leucyl-phenylalanine, phorbol 12-myristate 13-acetate (PMA), myelin basic protein, kinase A peptide inhibitor, protein A-Sepharose, and general reagents for kinase assays were from Sigma. [␥-32 P]ATP (specific activity 4000 Ci/mmol) was obtained from Bresatec, Adelaide, Australia. The anti-ERK antibody, R2, was a kind gift from Dr. S. Pelech, University of British Columbia, or was purchased from Upstate Biotechnology, Inc., Lake Placid, NY. Rabbit anti-p38 and anti-JNK1 antibodies were obtained from Santa Cruz Biotech. The anti-ACTIVE TM ERK and p38 antibodies were obtained from Promega Inc., Santa Cruz, CA. Enhanced chemiluminescence (ECL) solutions and reinforced nitrocellulose were from NEN Life Science Products and Schleicher and Schuell, respectively. Glutathione-Sepharose beads was from Pharmacia Biotech, Australia. Fatty acids, PMA, and formyl-methionyl-leucyl-phenylalanine were dissolved in ethanol, dimethyl sulfoxide (Me 2 SO), and Me 2 SO, respectively. The final concentrations of the vehicles were: ethanol, 0.1% (v/v) and Me 2 SO, 0.1% (v/v). Control cells received vehicle(s) alone.

Cell Culture
HeLa cells were maintained in Dulbeco's modified Eagle's medium in the presence of fetal calf serum (10%) and antibiotics as described previously (21). Cells (0.25 ϫ 10 6 ) were plated in 10-cm culture dishes and were used after 4 days. HL60 and Jurkat T cells were maintained in RPMI 1640 supplemented fetal calf serum with and antibiotics at Յ1 ϫ 10 6 /ml. All cells were washed once with Hanks' balanced salts solution (HBSS) 30 min before being incubated with 20:46 or vehicle.

Isolation and Incubation of Neutrophils
Human neutrophils were isolated from the peripheral blood of healthy volunteers by the rapid single-step method of Ferrante and Thong (22). The preparation of neutrophils was of Ͼ98% purity and Ͼ99% viability as judged by morphological examination of cytospin preparations and the ability of viable cells to exclude trypan blue. Cells in HBSS were incubated in the presence of 20:46 for the times indicated.

Preparation of Cellular Extracts
Incubations were terminated by removing the incubation medium and washing the cells once with HBSS (4°C).
After a 30-min incubation on ice, samples were centrifuged (100,000 ϫ g, 30 min), the supernatant was mixed with Laemmli buffer, and PKC isozymes were separated by SDS-polyacrylamide gel electrophoresis and immunoblotted with isozyme-specific anti-PKC antibodies as described below.
Kinase Assays p38 -p38 was immunoprecipitated before determination of kinase activity. Briefly, lysates (700 g of protein) were precleared with protein A-Sepharose (15 l/sample). Anti-p38 antibody (3 g/sample) was added, and tubes were incubated with constant mixing for 90 min at 4°C. The antigen-antibody complexes were precipitated by the addition of protein A-Sepharose (20 l/sample). The immunoprecipitates were washed once with buffer A and once with assay buffer (20 mM Hepes, pH 7.2, 20 mM ␤-glycerophosphate, 3.8 mM p-nitrophenyl phosphate, 10 mM MgCl 2 , 1 mM dithiothreitol, 50 M Na 3 VO 4 , and 20 M ATP) at 4°C. The assay was started by adding 30 l of assay buffer (30°C) containing 10 Ci of ␥ 32 P-ATP, 3.8 mM p-nitrophenylphosphate, and 15 g of myelin basic protein. After 15 min, the assay was terminated by the addition of Laemmli buffer and boiling the samples for 5 min at 100°C. Phosphorylated myelin basic protein was resolved by 12% SDS-polyacrylamide gel electrophoresis and was detected and quantitated using an Instant Imager (Packard Instruments).
JNK-A solid phase assay was used to assay JNK activity as described previously (24). Briefly, glutathione S-transferase-jun (1-79) fusion protein was purified from bacterial lysates using glutathione-Sepharose beads at 4°C with gentle rocking. 1 mg of lysate protein, 15 mM MgCl 2 , and 10 M ATP were added to 25 l (packed volume) of glutathione S-transferase-jun (1-79) coupled to glutathione-Sepharose beads. The mixtures were incubated for 2 h at 4°C with gentle rocking. After centrifugation (16,000 ϫ g, 5 min), the beads were washed once with buffer A, once with wash buffer (10 mM Pipes, pH 7, 100 mM NaCl, and the protease inhibitors, which were added to buffer A) and once with assay buffer (see p38 above). The assay was started by adding 35 l assay buffer containing 8 Ci of ␥ 32 P-ATP and bringing the temperature to 30°C. After 20 min, the assay was terminated by the addition of Laemmli buffer and boiling the samples for 5 min at 100°C. Samples were resolved by 10% SDS-polyacrylamide gel electrophoresis, and detection and quantitation of phosphorylated glutathione S-transferase-jun (1-79) was as described above.
ERK-ERK activity was assayed as described previously (12,23) by monitoring the incorporation of 32 P i into myelin basic protein in the presence of EGTA and protein kinase A peptide inhibitor. The assay mixture did not contain added phospholipids. Assays were terminated by spotting aliquots of the reaction mixture onto P81 filter paper. After 3 washes (5 min each) with 75 mM orthophosphoric acid, radioactivity associated with the paper was determined by liquid scintillation spectrometry. There was no detectable protein kinase A activity in phenyl-Sepharose-purified fractions, since omission of the protein kinase A peptide inhibitor from the assay mixture did not result in increased phosphorylation of myelin basic protein (Ref. 23 and data not shown). Active p38, if present in the fractions, was unlikely to contribute to any significant degree toward the total myelin basic protein kinase activity because the time course of ERK activity did not correlate with the appearance of dual-phosphorylated p38 (see "Results"). Consequently, it is unlikely that PKC, Ca 2ϩ /calmodulin-dependent kinases, p38, or protein kinase A were responsible for phosphorylating myelin basic protein in these samples.

Western Blotting
Denatured proteins were separated on either 10 (ERK and p38) or 12% (PKC) polyacrylamide gels and transferred to nitrocellulose (100 V, 1.5 h), and immunoreaction and detection were carried out as described earlier (25). Immediately after transfer, blots were stained with Ponceau S (0.1% in 5% acetic acid) to confirm equal loading of all lanes of the gels. Affinity-purified polyclonal anti-ERK antibody, R2, anti-AC-TIVE TM ERK, or anti-ACTIVE TM p38 antibody and anti-PKC isozymespecific antibodies were used to detect ERK isoforms, dual-phosphorylated ERK, dual phosphorylated p38, and PKC isozymes, respectively. Immunocomplexes were detected by enhanced chemiluminescence (25).

Statistical Analysis
Where appropriate, differences were analyzed by analysis of variance or unpaired Student's t test and were considered significant when p Ͻ 0.05.

RESULTS
Incubation of HeLa cells, HL60 cells, and human neutrophils with 20:46 (20 M) for 4 min resulted in the dual phosphorylation of p38 as detected by Western blotting (Fig. 1). Similar results were obtained in human umbilical vein endothelial cells (data not shown). Ponceau S staining confirmed that, within a particular experiment, the individual lanes were loaded with equal amounts of proteins (data not shown). Since the anti-ACTIVE™ p38 antibody only detects p38 that had been dual phosphorylated on the TGY activation motif, these results indicate activation of p38 by 20:46. Kinase activity assays in neutrophils confirmed this (Fig. 1). In contrast to the above data, 20:46 did not enhance p38 dual phosphorylation in Jurkat cells (data not shown) that express p38 (26).
Our previous studies in human neutrophils have demonstrated that 20:46 stimulated superoxide production, degranulation, and adherence to plastic surfaces and increased the expression of CD11b/CD18 (5-7). To elucidate the mechanisms through which 20:46 exerted these actions, the effects of 20: 46 on MAP kinases were studied in more detail in the neutrophils. 20:46 stimulated the dual phosphorylation of p38 in a concentration-and time-dependent manner (Fig. 2). Thus, dual-phosphorylated p38 could be detected at 5 M 20:46, and phosphorylation increased with increasing concentrations of 20:46 up to 20 M, the maximum concentration tested (Fig.  2a). Stimulation of p38 dual phosphorylation, detectable at less than 2 min, was transient, peaking at 5 min after exposure to 20:46 (Fig. 2b). Very little dual-phosphorylated p38 was left at 10 min after the addition of 20:46. The ability of 20:46 to stimulate dual phosphorylation of p38 was not diminished by either nordihydroguaiaretic acid, a broad spectrum inhibitor of the 5-, 12-, and 15-lipoxygenase or by indomethacin, an inhibitor of cyclooxygenase (Fig. 3). A small amount of dual-phosphorylated p38 was detected in neutrophils that had been exposed to either nordihydroguaiaretic acid or indomethacin per se. This was likely to be due to the accumulation of low levels of endogenous 20:46 in the presence of nordihydroguaiaretic acid or indomethacin.
We next examined whether 20:46 also stimulated the activity of JNK in human neutrophils. Although 20:46 has been reported to stimulate the activity of JNK in stromal and rabbit proximal tubular epithelial cells (19,20), the fatty acid did not stimulate JNK activity in neutrophils (data not shown). This was not because neutrophils do not express JNK, because the presence of JNK1 was detected in neutrophils (data not shown). However, 20:46 stimulated the activity of JNK in Jurkat T cells (Fig. 4), although the degree of activation was less than that observed with A23187/PMA (Fig. 4). 3 fatty acids also stimulated JNK activity in Jurkat cells (data not shown).
Although we have previously demonstrated that 20:46 stimulated the activity of ERK in WB rat liver cells (12), the effect of 20:46 on ERK activity in neutrophils has not been reported. Because the above data demonstrate that 20:46 stimulated the dual phosphorylation of p38 and the activity of JNK in a cell type-specific manner, it is, therefore, important to determine whether the activity of ERK in neutrophils is affected by 20:46. Activated ERK isoforms display reduced electrophoretic mobility in SDS-polyacrylamide gels (12,21,25,27)  ( Fig. 5a), consistent with their activation by phosphorylation. When the fractions were Western-blotted with anti-ACTIVE TM ERK antibody that detects active, dual-phosphorylated ERK, two bands with M r values of approximately 43-and 44-kDa were detected predominantly in samples from 20:46-stimulated cells (Fig. 5b). Kinase assays demonstrate that the enhancement of ERK activity by 20:46 was concentration-dependent. An increase in kinase activity was detectable at 5 M 20:46, the lowest concentration tested (Fig. 6a). The effect of 20:46 peaked at around 15 min after the addition of 20:46 (Fig. 6b) and was longer lasting than stimulation of p38 dual phosphorylation or activity (Fig. 2b). This argues strongly against the possibility that contaminating p38, which also phosphorylates myelin basic protein (Fig. 1b), was responsible for phosphorylating myelin basic protein in these fractions, since the appearance of dual-phosphorylated p38 peaked at 5 min after the addition of 20:46 and declined rapidly thereafter. 20:46 also stimulated the activity of ERK in human umbilical vein endothelial cells, human mesangial cells, Jurkat cells, HL60 cells, and human monocytes but not in PC12 pheochromocytoma cells (data not shown). The activity of ERK in these cells was also stimulated by the 3 fatty acids, eicosapentaenoic acid (20:53) and docosahexaenoic acid (22:63) (data not shown).
Since polyunsaturated fatty acids have been demonstrated to activate PKC in vitro (2, 3) and to stimulate the translocation of PKC in WB rat liver epithelial cells (12), we investigated whether PKC was involved in the activation of the p38 and ERK cascades by 20:46 in neutrophils. Neutrophils contain PKC ␣, ␤I, ␤II, ␦, and (28). Although polyunsaturated fatty acids have been reported to stimulate Ca 2ϩ mobilization (29), activate the neutral sphingomyelinase (30), and amplify H ϩ ion channel conductance (31) in intact neutrophils and to stimulate GTP␥S loading of the heterotrimeric G-proteins in neutrophil membrane fractions (32), the effect of fatty acids on PKC translocation in neutrophils has not been reported. In unstimulated neutrophils, a substantial amount of PKC ␤II was detected in a particulate fraction, and this was increased after incubation with 20:46 (Fig. 7). The existence of particulate fractionassociated PKC in unstimulated cells has also been observed in the T lymphocyte cell line, CTLL-2 (33). 20:46 also caused a small amount of PKC ␣ and ␤I to associate with the particulate fraction (Fig. 7). Neither PKC ␦ nor was detected in the particulate fraction (data not shown). An involvement of PKC in the activation of MAP kinases by 20:46 was confirmed by the observation that GF109203X, an inhibitor of classical PKC isozymes (34), attenuated the stimulatory effect of 20:46 on ERK activity by Ͼ85% (Fig. 8a). GF109203X also caused a modest reduction in the ability of 20:46 to stimulate the appearance of dual-phosphorylated p38 (Fig. 8b). DISCUSSION 20:46 is a second messenger molecule that is liberated from the sn-2 position of membrane phospholipids by ligand-stimulated activation of the cytosolic phospholipase A 2 (1). The importance of endogenously generated 20:46 in ligand-stimulated responses has been adequately demonstrated using inhibitors of cytosolic phospholipase A 2 and antisense technology (1). The non-esterified 20:46 that is released has been found to be cell-associated as well as being released into the extracellular medium. Thus, many studies have assayed for the appearance of radiolabeled 20:46 in the extracellular medium as a measure of phospholipase A 2 activation (1,35,36). Although cell-associated 20:46 can directly serve as an endogenous second messenger and is a substrate for the lipoxygenases and cyclooxygenases, 20:46 that is released into the extracellular fluid has the potential to exert autocrine and paracrine effects. Consistent with this suggestion, exogenously added The present study demonstrates that exogenous 20:46 stimulated the dual phosphorylation of p38 in HeLa cells, HL60 cells, human neutrophils, and human umbilical vein endothelial cells but not in Jurkat cells. We demonstrate in neutrophils that this increase in p38 dual phosphorylation was accompanied by an increase in p38 kinase activity. Stimulation of p38 dual phosphorylation by 20:46 in neutrophils was independent of its metabolism by either lipoxygenase or cyclooxygenase since the effect was not affected by nordihydroguaiaretic acid, a broad spectrum inhibitor of the 5-, 12-, and 15-lipoxygenases or by indomethacin, an inhibitor of cyclooxygenase. The fatty acid also stimulated the dual phosphorylation and activity of ERK but not of JNK in neutrophils. This, therefore, excludes an involvement of JNK in the actions of 20:46 in the neutrophils. However, 20:46 stimulated the activity of JNK in Jurkat T cells, an observation that is consistent with reports in proximal tubular epithelial cells and stromal cells that the activity of JNK was stimulated by 20:46 (19,20). The ability of 20:46 to stimulate the activity of ERK in human neutrophils and a number of other primary cell types and cell lines is consistent with our previous observations in WB rat liver epithelial cells (15). However, 20:46 did not affect the activity of ERK in PC12 cells, although ERK activity in these cells was strongly stimulated by PMA. 2 These data, therefore, demonstrate that 20:46 stimulated the activity of MAP kinases in a cell type/line-specific manner.
The present study demonstrates that PKC may be involved, at least in part, in mediating the effects of 20:46 on p38 and ERK activation. Thus, 20:46 not only stimulated the translo-cation of PKC ␣, ␤I, and ␤II to a particulate fraction in neutrophils, but the effects of 20:46 on p38 dual phosphorylation and ERK activity were attenuated by the PKC inhibitor, GF109203X. Consistent with a possible involvement of PKC in the p38 and ERK cascades, PMA, a direct activator of PKC, stimulates the activity of ERK in all cell types examined (18) and of p38 in some cell types (39,40). Recent studies have revealed that at least four members of the p38 family exist. These are p38␣ (also known as p38, CSBP, RK), p38␤, p38␥ (ERK6/SAPK3), and p38␦ (SAPK4) (41,42). PMA selectively stimulated the activity of p38␥ and p38␦ without significantly affecting the activity of p38␣ or p38␤ (42), indicating that the ␥ and ␦ forms of p38 are regulated by PKC. It remains to be determined whether the PMA-responsive p38 in neutrophils (39) and U937 cells (40) are p38␥ and/or p38␦. Although PKC may regulate the ERK cascade by direct phosphorylation of raf-1 (43) or via Shc/Ras (44), it is currently not known how PKC may regulate the p38 cascade.
In contrast to its effect on ERK activity, the effect of GF109203X on p38 dual phosphorylation was partial. This could imply that PKC is not the sole upstream regulator of the p38 cascade. 20:46 has been reported to stimulate the release of rho-GDI from its complex with rac2. guanine nucleotide dissociation inhibitor (45), and constitutively active rac has been found to stimulate the activity of p38 via p21-activated kinase (46). Hence, the fatty acid may also activate p38 via modulation of rac2 and p21-activated kinase, independently of PKC. Alternatively, the partial inhibition could suggest the possibility that neutrophils express both PKC-dependent and independent p38 forms. Until specific antibodies to p38 subtypes become available commercially, it is not possible to determine which p38 form(s) is activated by 20:46.
Although GF109203X has been generally regarded as a specific PKC inhibitor, a recent study has found that GF109203X also inhibited the activity of MAP kinase activated protein kinase-1␤ (rsk-2) and p70 S6 kinase (47). However, the effects of GF109203X on 20:46-stimulated ERK activity and p38 dual phosphorylation were unlikely to be due to inhibition of rsk-2 or p70 S6 kinase, since neither of these kinases are upstream regulators of ERK or p38.
The inability of 20:46 to stimulate JNK activity in neutrophils is in direct contrast to the observations in stromal (20) and proximal tubular epithelial cells (19). Although 20:46 stimulated the activity of JNK in Jurkat cells, this effect was weak compared with that caused by A21387 and PMA. Our failure to detect JNK activity was not because of a lack of JNK expression in neutrophils. Studies in proximal tubular epithelial cells have shown that stimulation of JNK activity by 20:46 requires activation of the NADPH oxidase (19). Given that 20:46 strongly stimulates the NADPH oxidase in neutrophils, it is, therefore, surprising that the fatty acid failed to stimulate the activity of JNK in neutrophils. This result clearly demonstrates that generation of oxygen radicals per se is insufficient to stimulate the JNK cascade.
Many ligands that stimulate the activity of MAP kinases also stimulate the activity of cytosolic phospholipase A 2 . It has been widely reported that ERK or p38 directly phosphorylates cytosolic phospholipase A 2 in activated cells and in in vitro assays (48,49) and, with the exception of thrombin-stimulated platelets (50), ERK or p38 has been found to directly regulate the enzymatic activity of cytosolic phospholipase A 2 . Our study, therefore, suggests that fatty acids such as 20:46, which are liberated by ligand-stimulated cytosolic phospholipase A 2, may participate in sustaining/amplifying MAP kinase activity and the activity of cytosolic phospholipase A 2 . Consistent with this, exogenously added polyunsaturated fatty acids have been 2 C. S. T. Hii and A. Ferrante, unpublished data. found to stimulate the activity of cytosolic phospholipase A 2 in intact neutrophils. 3 It is currently not clear how fatty acids are taken up into cells and exert their effects. There is evidence that indicates that fatty acids enter cells by simple diffusion (51) and/or via a carrier-mediated process. Proteins that function as fatty acid transporters have been reported to exist on the plasma membrane of a number of cell types (52,53). It is possible that these mechanisms are not mutually exclusive. Clearly, partititioning of a fatty acid into the plasma membrane per se is insufficient to exert a biological action (54,55). A detergent-like action of polyunsaturated fatty acids on the neutrophils has been excluded at concentrations that were used in this study (56). It is also unlikely that the biological activities of a fatty acid are dependent on esterification into membrane phospholipids, since the effects of fatty acids are reversed after the addition of delipidated serum albumin (4,29) too rapidly to support an esterification-based mechanism of action. A direct agonist-like fatty acid action is therefore likely.
The present study establishes for the first time that 20:46 stimulates the dual phosphorylation of p38 MAP kinase and that this stimulation is cell type-specific. Although this effect was observed in HeLa cells, HL60 cells, human umbilical vein endothelial cells, and human neutrophils, 20:46 did not increase the amount of dual-phosphorylated p38 in Jurkat T cells. Our studies also demonstrate that 20:46 stimulates the activity of ERK and JNK. Again, this effect was cell typespecific. Our data, therefore, suggest that ERK, p38, JNK, and PKC are potential mediators of the biological actions of 20:46. The MAP kinase species that is recruited will depend on the cell type.