Luo W, Sharif T R, Houghton P J, Sharif M
Department of Molecular Pharmacology, St. Jude Children's Research Hospital, Memphis, Tennessee 38105, USA.
Cell Growth Differ. 1997 Nov;8(11):1225-40.
The substance P (SP) receptor (NK-1 subtype) is widely expressed in primary human astrocytomas and glioblastomas and many brain tumor-derived cell lines. SP receptor activation stimulates the mitogen-activated protein (MAP) kinase pathway and the expression of immediate-early genes (e.g., c-Fos and c-Myc), resulting in an increase in DNA synthesis in human astrocytoma U-373 MG cells. In this study, we investigated the role of protein kinase C (PKC) in SP receptor activation of the MAP kinase pathway. SP peptide, epidermal growth factor, and the PKC activator 12-O-tetradecanoylphorbol-13-acetate (TPA) induced the tyrosine phosphorylation of the Erk1 and Erk2 MAP kinases in a concentration-dependent manner in U-373 MG cells. Pretreatment of the cells with PKC inhibitors, CGP 41251 or tamoxifen, inhibited tyrosine phosphorylation of Erk1 and Erk2 MAP kinases induced by low concentrations of SP or TPA and significantly attenuated phosphorylation at high concentrations of SP or TPA. The inhibitory effect exhibited by tamoxifen on SP-induced MAP kinase activation is similar to that exhibited by the selective PKC inhibitor CGP 41251, suggesting that the PKC enzyme is the in situ target for both inhibitors. Furthermore, SP-induced c-Fos phosphoprotein expression is inhibited by CGP 41251 or tamoxifen with similar efficacy. Importantly, neither CGP 41251 nor tamoxifen has any detectable effect on the MAP kinase activation by epidermal growth factor, consistent with the ability of this growth factor to activate the MAP kinase pathway by a PKC-independent mechanism. Prolonged treatment with TPA resulted in down-regulation of PKC and selective inhibition of TPA- and SP-induced Erk1 and Erk2 tyrosine phosphorylation in U-373 MG cells. Consistent with the in situ results, CGP 41251 and tamoxifen significantly inhibited endogenous PKC enzymatic activity from U-373 MG cells in vitro. In contrast to CGP 41251 and tamoxifen, Gö 6976, a highly selective inhibitor for PKC alpha and PKC beta 1 isozymes, did not inhibit SP- or TPA-induced tyrosine phosphorylation of Erk1 and Erk2 MAP kinases; rather, it inhibited a signaling pathway leading to the phosphorylation of cAMP-responsive element binding protein in U-373 MG cells. To investigate whether selective PKC isozyme(s) are involved in the activation of the MAP kinase pathway by SP, we determined the expression of PKC isozymes in U-373 MG cells. We found that U-373 MG cells express nine different PKC isozymes (alpha, beta I, beta II, epsilon, delta, eta, zeta, iota, and mu) and that stimulation with SP results in significant and selective translocation of PKC epsilon isozyme from cytosolic to membrane fraction. This establishes a correlation between the ability of SP to activate the MAP kinase pathway and its ability to translocate PKC epsilon. In conclusion, the results presented in this study demonstrate that SP receptor activation of PKC, possibly PKC epsilon, leads to the activation of the MAP kinase pathway, and that this pathway can be inhibited by known PKC inhibitors.
P物质(SP)受体(NK-1亚型)在原发性人类星形细胞瘤、胶质母细胞瘤以及许多脑肿瘤衍生细胞系中广泛表达。SP受体激活可刺激丝裂原活化蛋白(MAP)激酶途径以及即刻早期基因(如c-Fos和c-Myc)的表达,从而导致人星形细胞瘤U-373 MG细胞中DNA合成增加。在本研究中,我们调查了蛋白激酶C(PKC)在SP受体激活MAP激酶途径中的作用。SP肽、表皮生长因子以及PKC激活剂12-O-十四酰佛波醇-13-乙酸酯(TPA)在U-373 MG细胞中以浓度依赖性方式诱导Erk1和Erk2 MAP激酶的酪氨酸磷酸化。用PKC抑制剂CGP 41251或他莫昔芬预处理细胞,可抑制低浓度SP或TPA诱导的Erk1和Erk2 MAP激酶的酪氨酸磷酸化,并显著减弱高浓度SP或TPA时的磷酸化。他莫昔芬对SP诱导的MAP激酶激活的抑制作用与选择性PKC抑制剂CGP 41251的抑制作用相似,表明PKC酶是这两种抑制剂的原位靶点。此外,CGP 41251或他莫昔芬以相似的效力抑制SP诱导的c-Fos磷酸蛋白表达。重要的是,CGP 41251和他莫昔芬对表皮生长因子激活的MAP激酶均无任何可检测到的影响,这与该生长因子通过不依赖PKC的机制激活MAP激酶途径的能力一致。用TPA长期处理导致U-373 MG细胞中PKC下调,并选择性抑制TPA和SP诱导的Erk1和Erk2酪氨酸磷酸化。与原位结果一致,CGP 41251和他莫昔芬在体外显著抑制U-373 MG细胞的内源性PKC酶活性。与CGP 41251和他莫昔芬不同,Gö 6976是PKCα和PKCβ1同工酶的高度选择性抑制剂,它不抑制SP或TPA诱导的Erk1和Erk2 MAP激酶的酪氨酸磷酸化;相反,它抑制了U-373 MG细胞中导致cAMP反应元件结合蛋白磷酸化的信号通路。为了研究是否有选择性PKC同工酶参与SP对MAP激酶途径的激活,我们测定了U-373 MG细胞中PKC同工酶的表达。我们发现U-373 MG细胞表达九种不同的PKC同工酶(α、βI、βII、ε、δ、η、ζ、ι和μ),并且用SP刺激会导致PKCε同工酶从胞质部分向膜部分发生显著且选择性的转位。这确立了SP激活MAP激酶途径的能力与其使PKCε转位的能力之间的相关性。总之,本研究结果表明,SP受体激活PKC(可能是PKCε)会导致MAP激酶途径的激活,并且该途径可被已知的PKC抑制剂抑制。
