ABSTRACT
Zedoary tumeric (Curcumae Rhizoma, Ezhu in Chinese) has a long history of application and has great potential in the treatment of liver cancer. The antiliver cancer effect of zedoary tumeric depends on the combined action of multiple pharmacodynamic substances. In order to clarify the specific mechanism of zedoary tumeric against liver cancer, this paper first analyzes the mechanism of its single pharmacodynamic substance against liver cancer, and then verifies the joint anti liver cancer mechanism of its “pharmacodynamic group”. By searching the research on the antihepatoma effect of active components of zedoary tumeric in recent years, we found that pharmacodynamic substances, including curcumol, zedoarondiol, curcumenol, curzerenone, curdione, curcumin, germacrone, β-elemene, can act on multi-target and multi-channel to play an antihepatoma role. For example, curcumin can regulate miR, GLO1, CD133, VEGF, YAP, LIN28B, GPR81, HCAR-1, P53 and PI3K/Akt/mTOR, HSP70/TLR4 and NF-κB. Wnt/TGF/EMT, Nrf2/Keap1, JAK/STAT and other pathways play an antihepatoma role. Network pharmacological analysis showed that the core targets of the “pharmacodynamic group” for anti-life cancer are AKT1, EGFR, MAPK8, etc, and the core pathways are neuroactive live receiver interaction, nitrogen metabolism, HIF-1 signaling pathway, etc. At the same time, by comparing and analyzing the relationship between the specific mechanisms of pharmacodynamic substance and “pharmacodynamic group”, it is found that they have great reference significance in target, pathway, biological function, determination of core pharmacodynamic components, formation of core target protein interaction, in-depth research of single pharmacodynamic substance, increasing curative effect and so on. By analyzing the internal mechanism of zedoary tumeric pharmacodynamic substance and “pharmacodynamic group” in the treatment of liver cancer, this paper intends to provide some ideas and references for the deeper pharmacological research of zedoary tumeric and the relationship between pharmacodynamic substance and “pharmacodynamic group”.
ABSTRACT
OBJECTIVE:To study the effects of chitosan graphene oxide car rier(CS-GO)loaded with oridonin (CS-GO- oridonin)on the proliferation and apoptosis of human lung cancer A 549 cells. METHODS :Taking A 549 cells as objects ,the survival rate of cells were detected by CCK- 8 method after treated with different concentrations of CS-GO (3,6,12,24,48 μg/mL)and CS-GO-oridonin loaded with same mass of oridonin (3,6,12,24,48 μg/mL,by the weight of oridonin ,the same below). IC 50 of CS-GO-oridonin was calculated. The cell morphology were observed by microscope after treated with CS-GO and CS-GO-oridonin(both 32 μg/mL)for 2,4,10,24 h. The uptake of CS-GO ,oridonin,CS-GO-orionin(all 32 μg/mL)by cells was observed with fluorescence labeling method. The apoptosis of cells and the content of ROS were observed by flow cytometry after treated with different concentrations of CS-GO (16,32,64 μg/mL)and CS-GO-oridonin (16,32,64 μg/mL). The expression of anti-apoptosis related proteins (Mcl-1,Bax and Bak )were detected by Western blot. RESULTS :After treated with different concentrations of CS-GO ,the survival rate of cells was still above 90% ;after treated with different concentrations of CS-GO-oridonin,the survival rate of cells showed a downward trend ,and was significantly lower than that of CS-GO group (P< 0.01);IC50 of CS-GO-oridonin was 32.61 μg/mL. After CS-GO treatment,the cell morphology did not change significantly ;after CS-GO-oridonin treatment ,the cells shrunk and fell off in clusters ,and the suspended matter increased ;the fluorescence of oridonin and CS-GO-orionin taken up by cells was enhanced than CS-GO. Compared with blank group ,there was no significant change in the apoptosis rate ,the content of ROS and the expression of apoptosis-related protein in 16,32,64 μg/mL CS-GO groups(P>0.05);apoptosis rate ,the content of ROS ,the protein expression of Bax and Bak in 16,32,64 μg/mL CS- GO-oridonin groups were increased significantly ,while the protein expression of Mcl- 1 were decreased significantly. Above indexes were significantly high er or lower than the same concentration CS-GO group (P<0.05). CONCL USIONS:CS-GO dose not affect the proliferation and apoptosis of A 549 cells;CS-GO-oridonin has obvious inhibition and apoptosis promoting effect on cells ,which may be related to increasing ROS production and regulating the expression of apoptosis related proteins.