Accumulated evidence indicates that LPS-treated macrophage-induced COX-2 expression results in increased generation of prostaglandin E2 (PGE2). As a pro-inflammatory factor, PGE2 will ultimately leads to redness, swelling, heat, and pain. Previously, our laboratory has discovered the induction of c-Src in macrophages upon LPS exposure, which might contribute to macrophage migration and the secretion of TNFa. In this study, we demonstrated that LPS-mediated c-Src induction and migration were both abrogated in macrophage pre-treated with NS-398 (COX-2 inhibitor), implicating the involvement of PGE2 in macrophage activation. Intriguingly, while there was no alteration of the expression of the myeloid-specific SFKs (Hck, Lyn, and Fgr), upregulation of Src was detected in PGE2-stimulated Raw264.7 and rat peritoneal macrophage (PEMs). Elevated Src expression was participated in PGE2-induced macrophage mobility and TNFa secretion since PP2 could abolish all these effects. Remarkably, macrophages stimulated with dibutyryl adenosine (db-cAMP, a cAMP analogue) exhibited the similar results as those treated with PGE2, suggesting that cAMP was the second messenger in the signaling pathways initiated by PGE2. Notably, c-Src induction could also be detected in PEMs recovered from rats challenged with PGE2 and db-cAMP. Since H-89 (PKA inhibitor) could suppress PGE2-mediated c-Src induction and the concomitant macrophage migration and TNFa secretion, indicating the pathway: PGE2→AC→cAMP→PKA→Src. Due to LY294002 (PI3K inhibitor), PDTC (NF-kB inhibitor), PP2 (SFK inhibitor) could attenuate PGE2-mediated Src induction, it was likely that PI3K, NF-kB and SFK were also involved in this process.