LPS-induced activation of phospholipase A_2 phospholipase Cand protein kinase C of murine macrophage-like cell lines （J774 and P388D1）

A murine macrophage-like cell line,J774,acquried,in response to LPS,an ability to kill tumor necrosisfactor(TNF)-insensitive target P815 mastocytoma cells,whereas another cell line,P388D1,did not.LPS-triggered signaling mechanisms between the two celllines were compared with an aim to inquire about thepossible nature of the above-mentioned difference.Theresults showed that two cell lines respond to LPS-treatment by parallel activation of both phospholipasesC and A_2(PLC and PLA_2)to approximately the sameextent.The maximum response of both enzymes of J774cells was noted within 10 min of the treatment,whereas that of P388D1 cells required more than 20min.The other properties of LPS-responsive enzymesstudied were similar between two cell lines,ineludingActivation of PLC and PLA_2 and PKC in macrophages by LPSCa~(2 )augmentation of enzyme activation,participationof guanine nucleotide binding (G) proteins in theinitial activation processes,and inhibition of enzymeactivation by the prior treatment of cells with choleraorpartussis toxins etc.Moreover,LPS-triggered activationof PLC and PLA2 was found to be followed by theincrease of PKC activities in both cell lines.In spite ofthese similarities,J774 cells possessed both basic andacidic forms of PKC activities,while P 388D1 cells ownedonly PKC of basic form.Nevertheless,the question whyJ774 cells,but not P388D1 cells,can acquire thetumoricidal actiyity,aganist P815 cells following LPS-treatment remains to be answered.     

P48—Triggered transmembrane signaling transduction of human monocytes：modilization of calcium ion and activation of protein kinase C（PKC）

P48 is a cytokine which induces monocyte differentiation and the induction of cytotoxic activity.In this study,the signal transduction events involved in the stimulation of monocytes with the membrane form of P48 (mP48) were investigated.Monocyte stimulation with mP48 was found to involve the mobilization of intracellular calcium(Ca^2 ) and the activation and translocation of PKC from the cytosol to the membrane.Membane P48 induced a rapid rise of intracellular Ca^2 in a dose dependent maner.Similarly,the stimulation of monocytes with P48 was found to involve the activation and translocation of PKC.The translocation of PKC was rapid(within 0-5min) yet transient with PKC activity returning to control levels by 8 min.The functional role of protein kineses in P48 induced TNF secretion was studied using various kinese inhibitors.The PKC inhibitors,H-7 and sphingosine,were found to inhibit P48 induced TNF secretion with 50% inhibition at 5μM.HA1004,which inhibts cyclic nucleotide-dependent kinase(PKA,Ki 1.2μM),did not inhibit TNF secretion.H-8(PKA inhibitor) was found to be an effective inhibitor of TNF secretion only at high concentrations(30μM).The Calmodulin-dependent kinase inhibitor,W7(Ki 12μM) was found to be effective at concentration above 5μM.These findings suggest that P48-triggered TNF secretion involves transmembrane Ca^2 signaling and the subsequent activation of at least two protein kineses,PKC and CaMK.     

A cotton mitogen-activated protein kinase （GhMPK6） is involved in ABA-induced CAT1 expression and H2O2 production

The mitogen-activated protein kinase (MAPK) cascade is one of the major and evolutionally conserved signaling pathways and plays a pivotal role in the regulation of stress and developmental signals in plants.Here,we identified one gene,GhMPK6,encoding an MAPK protein in cotton.GFP fluorescence assay demonstrated that GhMAPK6 is a cytoplasm localized protein.Quantitative RT-PCR analysis revealed that mRNA accumulation of GhMPK6 was significantly promoted by abscisic acid (ABA).Overexpression of GhMPK6 gene in the T-DNA insertion mutant atmkkl (SALK_015914) conferred a wild-type phenotype to the transgenic plants in response to ABA.Under ABA treatment,cotyledon greening/expansion in GhMPK6 transgenic lines and wild type was significantly inhibited,whereas the atmkkl mutant showed a relatively high cotyledon greening/expansion ratio.Furthermore,CAT1 expression and H2O2 levels in leaves of GhMPK6 transgenic lines and wild type were remarkably higher than those of atmkkl mutant with ABA treatment.Collectively,our results suggested that GhMPK6 may play an important role in ABA-induced CAT1 expression and H2O2 production.