尿多酸肽抑制多发性骨髓瘤细胞株RPIMI 8226增殖及其机制研究

叶宝东; 邵科钉; 陈丹; 张翔; 张宇; 周郁鸿

引用本文:	叶宝东,邵科钉,陈丹,张翔,张宇,周郁鸿.尿多酸肽抑制多发性骨髓瘤细胞株RPIMI 8226增殖及其机制研究[J].中国现代应用药学,2013,30(11):1161-1165.
	YE Baodong,SHAO Keding,CHEN Dan,ZHANG Xiang,ZHANG Yu,ZHOU Yuhong.Uroacitides(CDA-2) Inhibited the Proliferation of Multiple Myeloma Cell Line RPMI 8226[J].Chin J Mod Appl Pharm(中国现代应用药学),2013,30(11):1161-1165.

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尿多酸肽抑制多发性骨髓瘤细胞株RPIMI 8226增殖及其机制研究
叶宝东, 邵科钉, 陈丹, 张翔, 张宇, 周郁鸿
浙江中医药大学附属第一医院，杭州 310006

摘要:

目的探讨尿多酸肽(CDA-2)抑制多发性骨髓瘤细胞株RPMI8226增殖作用及其机制。方法采用四甲基偶氮唑(MTT)比色法检测CDA-2对RPMI8226抑制作用并筛选研究浓度；通过Hoechst33258、Annexin-V/PI、细胞周期分析、DNA琼脂糖凝胶电泳等方法检测CDA-2诱导RPMI8226凋亡作用；使用Western Blot法检测caspase-8、caspase-3及其激活物的表达改变；半定量RT-PCR法检测TNF、FADD、TRAF3 mRNA表达。结果 CDA-2能够抑制RPMI8226细胞株增殖，并呈浓度依赖性，IC50为1.64 mg·mL^-1；经CDA-2作用后，Hoechst33258荧光染色提示细胞核浓集及出现凋亡小体，Annexin-V/PI分析示早期凋亡细胞比例呈时间依赖增加，细胞周期分析提示呈浓度依赖上调凋亡峰及下调G1期比例，DNA凝胶电泳可见断裂成180~200 bp及其倍数的片断梯形条带，故CDA-2可诱导RPMI8226细胞株凋亡；Western Blot检测发现随药物作用时间延长caspase-8、caspase-3表达明显下降，而active-caspase8、active-caspase3表达上升；半定量RT-PCR证实凋亡相关基因TNF、FADD、TRAF3 mRNA表达上调。结论 CDA-2可抑制RPMI8226增殖，且可通过死亡受体途径诱导细胞凋亡。

关键词: 尿多酸肽 RPMI8226 增殖抑制

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基金项目:浙江省“十二五”第一批省重中之重一级学科项目

Uroacitides(CDA-2) Inhibited the Proliferation of Multiple Myeloma Cell Line RPMI 8226

YE Baodong, SHAO Keding, CHEN Dan, ZHANG Xiang, ZHANG Yu, ZHOU Yuhong

The First Affiliated Hospital of Zhejiang Chinese Medicine University, Hangzhou 310006, China

Abstract:

OBJECTIVE To explore the effects of uroacitides(CDA-2) on the proliferation of RPMI 8226 cells and its mechanisms. METHODS The proliferative inhibition of CDA-2 on RPMI 8226 cells was detected by MTT and the drug concentrations for further researches were screened out. The apoptosis of RPMI8226 cells after treating with CDA-2 was analyzed by Hoechst33258 staining, Annexin-V/PI staining, PI staining, and DNA gel electrophoresis. Changes in the expression of caspase-8, caspase-3 and their active forms were tested by Western Blot. The expression of TNF, ADD and TRAF3 mRNA were detected by semi-quantitative RT-PCR. RESULTS CDA-2 inhibited the proliferation of RPMI8226 cells in a dose-dependent manner with the IC50 1.64 mg·mL^-1. Condensed nuclei and apoptotic body were found via Hoechst33258 fluorescence staining when cells were treated with CDA-2. Annexin-V/PI analysis showed that the proportion of early apoptotic cells raised in a time-dependent manner. Cell cycle analysis showed that the apoptotic peak was up-regulated and G1 phase was decreased in a dose-dependent manner. DNA gel electrophoresis revealed integer multiples of 180~200 bp “ladder” bands. Western blot revealed that the expression of caspase-8, caspase-3 was down-regulated, while the expression of active caspase-8, activecaspase-3 was increased as the exposed time extended. The semi-quantitative RT-PCR showed up-regulation of TNF, FADD, TRAF3 mRNA, which were associated with apoptosis. CONCLUSION CDA-2 inhibited the proliferation of RPMI8226 cells and induced apoptosis via death receptor pathway.

Key words: uroacitides(CDA-2) RPMI8226 proliferative inhibition