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作 者:梁钢[1] 张肃[1] 黄志明[1] 黄仁彬[1] 梁宁生[2] 许佐良[3]
机构地区:[1]广西医科大学药理学教研室,南宁530021 [2]广西医科大学附属肿瘤医院药剂科,南宁530021 [3]北京大学医学部临床肿瘤学院免疫室,北京100083
出 处:《中国天然药物》2004年第2期119-122,共4页
基 金:广西省科技厅自然科学基金资助项目 (桂科自No 0 0 0 43 0 2 )~~
摘 要:目的 :研究两种儿茶素成分ECG、EGCG是否对人耐药肝癌细胞BEL 74 0 4 /Adr和耐药口腔癌细胞KBV2 0 0存在细胞毒增敏作用及可能的机制。方法 :用MTT法检测药物对体外培养的细胞的毒性作用 ,用RT PCR法检测MDR1表达 ,流式细胞仪测定P gp表达及细胞内Rh 12 3含量。结果 :两种儿茶素成分在 10 0 μg·ml-1以下剂量对两株耐药肿瘤细胞的抑制率均小于 10 % ,6 0 μg·ml-1ECG或 14 μg·ml-1EGCG联合 0 8μg·ml-1ADM或 0 12 μg·ml-1VCR时MDR1下降 2 3 9%~ 38 6 % ,两种儿茶素成分与抗肿瘤药物联合应用可使P gp表达下降 ,能明显提高细胞内Rh 12 3的含量。结论 :儿茶素成分ECG、EGCG与ADM或VCR联合应用可增强耐药肿瘤细胞BEL 74 0 4 /Adr和耐药口腔癌细胞KBV2 0 0的细胞毒作用 ,其机制可能与降低MDR1 mRNA表达、下调P gp表达及抑制P gp的功能有关。AIM:To study the chemotherapy sensitizing effect of ECG and EGCG on human multidrug resistant cells BEL-7404/Adr and KBV200 and its possible mechanism.METHOD:MTT was used to test the cytotoxicity of drugs.MDR_ 1 expression was detected by RT-PCR.FACS was used to determine the expression of P-gp and the concentration of Rh123 in carcinoma cells.RESULT:Both of the cell inhibition rate of two catechin monomers are under 10% at the dose of less than 100 μg·ml -1 .MDR_ 1 expression was reduced at 23.9%~38.6% by 60 μg·ml -1 ECG or 14 μg·ml -1 EGCG combined with 0.8 μg·ml -1 ADM or 0.12 μg·ml -1 VCR.The combination also decreased the expression of P-gp and enhanced the concentration of Rh123 in carcinoma cells.CONCLUSION:ECG or EGCG combined with chemicals respectively could enhance the cytotoxicity of chemicals on BEL-7404/Adr or KBV200.The mechanism was possibly related to decreasing the expression of MDR_ 1 -mRNA,P-gp and inhibiting the function of P-gp.
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