Roles of PLC-γ2 and PKCα in TPA-induced apoptosis of gastric cancer cells

AIM: To investigate the roles of PLCγ2 and PKCα in TPA-induced apoptosis of gastric cancer cells.METHODS: Human gastric cancer cell line MGC80-3 was used. Protein expression levels of PLCγ2 and PKCα were detected by Western blot. Protein localization of PLCγ2 and PKCα was shown by immunofluoscence analysis under laserscanning confocal microscope. Apoptotic morphology was observed by DAPI fluorescence staining, and apoptotic index was counted among 1 000 cells randomly.RESULTS: Treatment of gastric cancer cells MGC80-3 with TPA not only up-regulated expression of PLC-γ2 protein,but also induced PLC-γ2 translocation from the cytoplasm to the nucleus. However, this process was not directly associated with apoptosis induction. Further investigation showed that PKCa translocation from the cytoplasm to the nucleus was correlated with initiation of apoptosis. To explore the inevitable linkage between PLC-γ2 and PKCα during apoptosis induction,PLC inhibitor U73122 was used to block PLC-γ2 translocation,in which neither stimulating PKCα translocation nor inducing apoptosis occurred in MGC80-3 cells. However, when U73122treated cells were exposed to TPA, not only PLC-γ2, but also PKCα was redistributed. On the other hand, when cells were treated with PKC inhibitor alone, PLC-γ2 protein was still located in the cytoplasm. However, redistribution of PLC-γ2 protein occurred in the presence of TPA, no matter whether PKC inhibitor existed or not.CONCLUSION: PLC-γ2 translocation is critical in transmitting TPA signal to its downstream molecule PKCα. As an effector,PKCα directly promotes apoptosis of MGC80-3 cells.Therefore, protein translocation of PLCγ2 and PKCα is critical event in the process of apoptosis induction.

佛波酯处理人胃癌MGC80-3细胞过程中磷酯酶C-γ2的意义

目的探讨佛波酯(TPA)处理人胃癌MGC80-3细胞过程中磷酯酶Cγ-2(PLCγ-2)的意义。方法通过DAPI染色,荧光显微镜观察分析TPA对胃癌MGC80-3细胞的影响;借助核浆分离手段获得胃癌细胞核浆蛋白,并通过免疫印迹(Western blotting)检测TPA对PLCγ-2蛋白表达水平影响;通过免疫荧光技术处理,激光扫描共焦显微镜观察胃癌细胞内PLCγ-2蛋白的定位和转运;用PLCγ-2的抑制剂(U73122)预处理细胞,免疫印迹和激光扫描共焦显微镜分别检测其对TPA作用胃癌细胞内PLCγ-2的影响;以及荧光显微镜下观察分析U73122是否影响TPA对胃癌细胞的作用。结果TPA诱导胃癌MGC80-3细胞凋亡;同时TPA提高PLCγ-2蛋白表达水平,并诱导其发生核浆转运;其抑制剂(U73122)可以降低TPA对PLCγ-2蛋白表达水平的作用,但并不能影响TPA诱导胃癌细胞凋亡;而TPA诱导的PLCγ-2核浆转运却没有被PLCγ-2抑制剂(U73122)阻止。结论尽管TPA提高了胃癌MGC80-3细胞中PLCγ-2表达水平,但PLCγ-2表达水平和TPA诱导的胃癌MGC80-3凋亡没有直接关系,而其核浆转运可能与TPA诱导的胃癌细胞凋亡相关。

枳术丸汤剂含药血清对大鼠结肠Cajal间质细胞增殖及PLC-γ信号通路的影响

目的探讨枳术丸治疗慢传输型便秘的可能作用机制。方法20只SD雄性大鼠随机分为枳术丸汤剂组、空白组,每组10只。枳术丸汤剂组大鼠每日给予浓度为2 g/ml枳术丸汤剂5.8 g灌胃,连续7天,空白组正常饲养。末次给药后1 h腹主动脉采血离心制备含药血清。采用CCK8法观察磷脂酶C-γ(PLC-γ)特异性抑制剂U73122对大鼠结肠原代Cajal间质细胞的细胞抑制率来筛选药物浓度,观察5%、10%、15%、20%浓度的枳术丸汤剂含药血清对Cajal间质细胞的细胞增殖率筛选药物浓度,并分别培养12、24、48 h来筛选用药时间。取二或三代Cajal间质细胞接种至96孔板中,每孔1×10^(4)个细胞,每组重复3孔。实验分为正常组、模型组(正常细胞+筛选浓度的U73122)、空白血清组(模型组+10%空白血清)、枳术丸汤剂血清组(模型组+筛选浓度枳术丸含药血清)。干预时间为实验筛选出的时间。免疫组化法检测磷脂酶C-γ1(PLC-γ1)、磷脂酶C-γ2(PLC-γ2)阳性表达,Western blot法检测PLC-γ1、PLC-γ2蛋白表达,RT-PCR法检测PLC-γ1、PLC-γ2基因表达。结果筛选出U73122最佳实验药物浓度为30μmol/L,枳术丸汤剂组最佳用药浓度为5%,实验最佳干预时间为24 h。与正常组比较,模型组PLC-γ1、PLC-γ2平均光密度值、蛋白及基因表达均降低(P<0.01);与模型组比较,枳术丸汤剂血清组、空白血清组PLC-γ1、PLC-γ2平均光密度值、蛋白及基因表达均升高(P<0.05或P<0.01);与空白血清组比较,枳术丸汤剂血清组PLC-γ1、PLC-γ2阳性表达、蛋白及基因表达明显增多(P<0.01)。结论枳术丸汤剂可能通过激活Cajal间质细胞PLC-γ信号通路,调控细胞增殖,从而促进胃肠运动。