Down-regulation of extracellular signal-regulated kinase 1/2 activity in P-glycoprotein-mediated multidrug resistant hepatocellular carcinoma cells

AIM： To study the expression and phosphorylation of extracellular signal-regulated kinase （ERK） i and ERK2 in multidrug resistant （MDR） hepatocellular carcinoma （HCC） cells.METHODS： MDR HCC cell lines, HepG2/adriamycin （ADM） and SMMC7721/ADM, were developed by exposing parental cells to stepwise increasing concentrations of ADM. MTT assay was used to determine drug sensitivity. Flow cytometry was employed to analyze cell cycle distribution and measure cell P-glycoprotein （P-gp） and multidrug resistant protein 1 （MRP1） expression levels. ERK1 and ERK2 mRNA expression lev-ls were measured by quantitative real-time PCR （QRTPCR）. Expression and phosphorylation of ERK1 and ERK2 were analyzed by Western blot.RESULTS： MTT assay showed that HepG2/ADM andSMMC7721/ADM were resistant not only to ADM, but also to multiple anticancer drugs. The P-gp expression was over 10-fold higher in HepG2/ADM cells than in HepG2 cells （8.92% ±0.22% vs 0.88% ± 0.05%, P 〈 0.001） and over 4-fold higher in SMMC7721/ADM cells than in SMMC7721 cells （7.37% ± 0.26% vs 1.74% ± 0.25%, P 〈 0.001）. However, the MRP1 expression was not significantly higher in HepG2/ADM and SMMC7721/ADM cells than in parental cells. In addition, the percentage of MDR HepG2/ADM and SMMC7721/ADM cells was significantly decreased in the G0/G1 phase and increased in the the S phase or G2/M phase. QRT-PCR analysis demonstrated that the ERK1 and ERK2 mRNA expression increased apparently in HepG2/ADM cells and decreased significantly in SMMC7721/ADM cells. Compared with the expression of parental cells, ERK1 and ERK2 protein expressions were markedly decreased in SMMC7721/ADM cells. However, ERK2 protein expression was markedly increased while ERK1 protein expression had no significant change in HepG2/ADM cells. Phosphorylation of ERK1 and ERK2 was markedly decreased in both HepG2/ADM and SMMC7721/ADM MDR cells.CONCLUSION： ERK1 and ERK2 activities are downregulated in P-gp-mediated MDR HCC cells. ERK1 or ERK2 might be a potential drug target for circumventing MDR HCC cells,

MGC803细胞中MAPK信号传导系统与MDR1关系的研究

目的:探讨在人胃癌细胞系MGC803中促分裂原激活的蛋白激酶(mitogen-activatedproteinkinase,MAPK)信号传导系统与MDR1基因表达的关系。方法:通过westernblot验证MGC803细胞在长春新碱(vincristine,VCR)作用下MDR1基因编码的P-糖蛋白(P-glycoprotein,P-gp)的表达及特异性MAPK抑制剂PD098059对P-gp表达的抑制,通过流式细胞术对VCR及PD098059作用下的细胞进行周期解析,同时用MTT法验证VCR诱导后及PD098059作用下的药物敏感性。结果:MGC803细胞在VCR短期作用下,P-gp表达增加,在PD098059的作用下其表达受到抑制。通过细胞的周期解析发现VCR和PD098059共同作用的细胞凋亡比例为35.61%,显著高于VCR单独作用引起的凋亡(18.41%)(P<0.05)。VCR刺激后MGC803细胞的IC50为284ng/ml,分别为阴性对照组(127ng/ml)的2.24倍,为VCR+PD098059组(191ng/ml)的1.48倍。结论:MGC803细胞在VCR的短期作用下可诱导产生P-gp,而PD098059可抑制P-gp的表达和逆转其耐药性,从而增加MGC803细胞的凋亡。MAPK有可能通过调节MDR1的转录和翻译而影响细胞的耐药性。

PKC抑制剂对MGC803细胞中P-gp表达及耐药性的影响

背景与目的:既往研究发现,肿瘤细胞的多药耐药(multidrugresistance,MDR)与蛋白激酶C(proteinkinaseC,PKC)信号转导系统关系密切,但其作用机制有待于进一步研究。本实验拟通过研究长春新碱(vincristine,VCR)及选择性PKCα、β抑制剂myr-ψPKC对人胃癌细胞MGC803的作用,探讨PKC信号转导系统与mdr1基因的关系。方法:用Westernblot检测MGC803细胞中mdr1基因编码的P-糖蛋白(P-glycoprotein,P-gp)的表达以及VCR作用对其表达的影响,用流式细胞术对VCR及作用后的细胞进行周期分析,同时用MTT法验证VCR诱导后及其作用下MGC803细胞的药物敏感性。结果:MGC803细胞在VCR短期作用下,P-gp表达增加,在myr-ψPKC的作用下其表达受到抑制。通过细胞周期分析发现VCR和myr-ψPKC共同作用的细胞其凋亡比例为31.23%,显著高于VCR单独作用时的细胞凋亡率(18.41%)(P<0.05)。VCR刺激后MGC803细胞对VCR的IC50为(284.0±13.2)ng/ml,是阴性对照组IC50犤(127.0±17.6)ng/ml犦的2.24倍,是myr-ψPKC组IC50犤(212.0±30.4)ng/ml犦的1.33倍。结论:MGC803细胞在VCR的短期作用下可诱导产生P-gp,而myr-ψPKC可通过选择性抑制PKCα、β而抑制P-gp的表达和逆转其耐药性,从而促进MGC803细胞的凋亡。PKC可能对胃癌mdr1表达有调节作用。

山奈酚逆转慢性粒细胞白血病K562/ADM细胞耐药性及相关机制

目的探讨山奈酚逆转耐多柔比星(ADM)的慢性粒细胞白血病K562/ADM细胞耐药性及相关机制。方法采用四甲基偶氮唑盐(MTT)法检测ADM作用24 h对K562和K562/ADM细胞的毒性,计算24 h ADM半数抑制浓度(IC50)及耐药倍数。MTT法检测山奈酚作用24 h对K562/ADM细胞的毒性,计算24 h山奈酚5%抑制浓度(IC5)、10%抑制浓度(IC10),以二者确定后续实验山奈酚两组浓度,未经山奈酚处理的细胞为空白对照组。采用MTT法检测空白对照组及山奈酚干预组ADM作用24 h的细胞抑制情况,计算各组24 h的细胞抑制情况,计算各组24 h ADM IC50,空白对照组与山奈酚组IC50的比值为山奈酚逆转耐药倍数。应用流式细胞术检测山奈酚作用后K562/ADM细胞内ADM荧光强度。采用蛋白质印迹法检测分别经山奈酚、p38-MAPK信号通路特异性抑制剂SB202190、山奈酚和SB202190联用后的K562/ADM细胞耐药蛋白[P糖蛋白(P-gp)、多药耐药相关蛋白1(MRP1)、磷酸化p38(p-p38)、总p38(t-p38)]表达情况。结果ADM处理24 h后,K562、K562/ADM细胞IC50值分别为(0.9±0.6)、(28.1±3.5)μg/ml;相对于K562细胞,K562/ADM细胞对ADM作用24 h的耐药倍数为31.16倍。MTT法检测结果显示,山奈酚呈剂量依赖性抑制K562/ADM细胞增殖,依据IC5和IC10,确定以0.5、1.0μmol/L山奈酚进行后续实验。山奈酚和ADM共同作用24 h后,空白对照组、0.5μmol/L山奈酚组、1.0μmol/L山奈酚组K562/ADM细胞24 h ADM IC50分别为(33.7±5.7)、(21.4±0.6)、(15.9±1.8)μg/ml(F=30.85,P<0.05;组内两两比较,均P<0.05),0.5μmol/L山奈酚组、1.0μmol/L山奈酚组K562/ADM细胞24 h逆转耐药倍数分别为1.58、2.12倍。流式细胞术检测示,空白对照组、0.5μmol/L山奈酚组、1.0μmol/L山奈酚组K562/ADM细胞内ADM平均荧光强度(MFI)分别为138.4±8.9、154.3±2.2、165.7±4.8,差异有统计学意义(F=161.48,P<0.05)。与空白对照组比较,0.5、1.0μmol/L山奈酚处理24 h后,K562/ADM细胞的P-gp、MRP1、p-p38蛋白相对表达量均降低(均P<0.05),而t-p38蛋白表达量差异无统计学意义(P>0.05);SB202190可降低P-gp、MRP1、p-p38蛋白的相对表达量(均P<0.05);SB202190联合不同浓度山奈酚作用后,K562/ADM细胞P-gp、MRP1、p-p38蛋白的相对表达量未下降(P>0.05)。结论山奈酚可能通过抑制p38-MAPK通路降低K562/ADM细胞P-gp、MRP1的相对表达量,实现增加细胞内ADM的蓄积,从而逆转K562/ADM细胞的耐药性。