摘要
Objective:Hederacolchiside A1,exhibits cytostatic and cytotoxic activity against various cancer cells in vitro,however,the mechanism is not well understood.Methods:In this study,hederacolchiside A1 from Pulsatilla chinensis was isolated and tested its anticancer activity and mechanism.Hederacolchiside A1 could inhibit proliferation of A549,SMMC-7721,BEL-7402,and MCF-7 cells by MTT assay.Investigations of apoptosis of treated cancer cells were identified in hederacolchiside A1 by flow cytometric analysis of annexin V expression.Results:Based on the results of western blotting and JC-1 staining,hederacolchiside A1 reduced the mitochondrial membrane potential and Bcl-2 protein levels,whereas cleaved caspase-3 was higher.Furthermore,hederacolchiside A1 effectively inhibited the phosphorylations of phosphatidylinositol 3 kinase(PI3K),protein kinase B(Akt),and mammalian target of rapamycin(m TOR).In vivo study showed that hederacolchiside A1(3.0,4.5,and 6.0 mg/kg,ip)could significantly inhibit the weight of tumor in anmodel.Similar inhibitory activities were observed when the compound(3.25,7.5,and15.0 mg/kg,ig)was tested in nude mice xenograft tumor models using human breast carcinoma MCF-7 cells.Conclusion:These data indicated that hederacolchiside A1 suppressed the proliferation of human tumor cells by inducing apoptosis through modulating the PI3K/Akt/m TOR signaling pathway.
Objective:Hederacolchiside A1,exhibits cytostatic and cytotoxic activity against various cancer cells in vitro,however,the mechanism is not well understood.Methods:In this study,hederacolchiside A1 from Pulsatilla chinensis was isolated and tested its anticancer activity and mechanism.Hederacolchiside A1 could inhibit proliferation of A549,SMMC-7721,BEL-7402,and MCF-7 cells by MTT assay.Investigations of apoptosis of treated cancer cells were identified in hederacolchiside A1 by flow cytometric analysis of annexin V expression.Results:Based on the results of western blotting and JC-1 staining,hederacolchiside A1 reduced the mitochondrial membrane potential and Bcl-2 protein levels,whereas cleaved caspase-3 was higher.Furthermore,hederacolchiside A1 effectively inhibited the phosphorylations of phosphatidylinositol 3 kinase(PI3K),protein kinase B(Akt),and mammalian target of rapamycin(m TOR).In vivo study showed that hederacolchiside A1(3.0,4.5,and 6.0 mg/kg,ip)could significantly inhibit the weight of tumor in anmodel.Similar inhibitory activities were observed when the compound(3.25,7.5,and15.0 mg/kg,ig)was tested in nude mice xenograft tumor models using human breast carcinoma MCF-7 cells.Conclusion:These data indicated that hederacolchiside A1 suppressed the proliferation of human tumor cells by inducing apoptosis through modulating the PI3K/Akt/m TOR signaling pathway.
基金
funded by the National Sciences Foundation of China(No.81273402,81573548)
