[小干扰RNA敲低MG-63细胞中细胞周期蛋白A2的表达]
[Knockdown of cyclin A2 expression by small interfering RNA in MG-63 cells].
作者信息
Liu Ye, Ding Jia-Yi, Shen Wei-Liang, Zhao Xing, Fan Shun-Wu
机构信息
Department of Orthopaedics, Sir Run Run shaw Hospital, Zhejiang University, Hangzhou 310016, China.
出版信息
Zhonghua Zhong Liu Za Zhi. 2007 Sep;29(9):670-5.
OBJECTIVE
To study the inhibitory effect of small interference RNA (siRNA) targeting cyclin A2 gene on the growth of osteosarcoma MG-63 and human normal skin fibroblast HSF cells and to explore whether cyclin A2 siRNAs could become a useful tool in the treatment of osteosarcoma.
METHODS
Three pairs of siRNAs targeting cyclin A2 mRNA and a pair of nonsense siRNA were designed according to the current criteria. SiRNAs were chemically synthesized and purified. The siRNAs were transfected into MG-63 cells and HSF cells via oligofectamine. The cells transfected with nonsense siRNA served as negative control group and those only treated with PBS as blank control group. Quantitative fluorescence RT-PCR, Western-blot, MTT assay, reverse transcriptase (RT)-PCR, flow cytometry and clone forming test were employed to evaluate the efficacy of RNA interference. At the same time, the mRNA expression of PCNA and cyclin B1 in siRNA-treated MG-63 cells were examined.
RESULTS
Although all three siRNAs could reduce the cyclin A2 expression, siRNA, appeared to be the most effective. After 48 h treatment with siRNA1, cyclin A2 mRNA and protein expression in MG-63 cells was significantly reduced by nearly 80% as compared with that of the blank control group, whereas the negative and blank control groups had similar expression levels. MG-63 cells treated with siRNA1 were arrested at G0/G1 phase by 80.1% and the proliferation of these tumor cells was suppressed 48 h after transfection. Furthermore, MG-63 cells showed a decreased colony forming ability after siRNA1 treatment. In addition, the cyclin A2-depleted MG-63 cells showed decreased levels of PCNA and cyclin B1. In contrast, although cyclin A2 expression in HSF reduced by nearly 60% after treatment by siRNA1 for 48h, these cells exhibited only a slight change in cell cycling, and neither clear inhibition of proliferation nor impaired colony forming ability was observed.
CONCLUSION
Cyclin A2 is critical for proliferation of MG-63 cells. Cyclin A2-siRNAs can induce obvious inhibition of cyclin A2 mRNA and protein expression in MG-63 and HSF cells, which consequently down-regulate the proliferation of MG-63 cells. There is little effect on the proliferation of siRNA-treated HSF cells. Those results indicate that siRNAs against cyclin A2 may become a potential antiproliferative tool in future antitumor therapy.
目的
研究靶向细胞周期蛋白A2(cyclin A2)基因的小干扰RNA(siRNA)对骨肉瘤MG-63细胞和人正常皮肤成纤维细胞HSF生长的抑制作用,并探讨cyclin A2 siRNAs能否成为治疗骨肉瘤的有效工具。
方法
根据现有标准设计3对靶向cyclin A2 mRNA的siRNAs和1对无义siRNA。化学合成并纯化siRNAs。通过脂质体转染试剂将siRNAs转染至MG-63细胞和HSF细胞。转染无义siRNA的细胞作为阴性对照组,仅用PBS处理的细胞作为空白对照组。采用定量荧光RT-PCR、Western-blot、MTT法、逆转录(RT)-PCR、流式细胞术和克隆形成试验评估RNA干扰的效果。同时,检测siRNA处理的MG-63细胞中增殖细胞核抗原(PCNA)和细胞周期蛋白B1(cyclin B1)的mRNA表达。
结果
尽管3种siRNAs均能降低cyclin A2的表达,但siRNA1似乎最为有效。用siRNA1处理48小时后,MG-63细胞中cyclin A2的mRNA和蛋白表达与空白对照组相比显著降低了近80%,而阴性对照组和空白对照组的表达水平相似。用siRNA1处理的MG-63细胞80.1%停滞于G0/G1期,转染后48小时这些肿瘤细胞的增殖受到抑制。此外,用siRNA1处理后MG-63细胞的克隆形成能力下降。另外,cyclin A2缺失的MG-63细胞中PCNA和cyclin B1的水平降低。相比之下,虽然用siRNA1处理48小时后HSF细胞中cyclin A2的表达降低了近60%,但这些细胞的细胞周期仅出现轻微变化,未观察到明显的增殖抑制和克隆形成能力受损。
结论
Cyclin A2对MG-63细胞的增殖至关重要。Cyclin A2-siRNAs可显著抑制MG-63和HSF细胞中cyclin A2的mRNA和蛋白表达,从而下调MG-63细胞的增殖。对经siRNA处理的HSF细胞的增殖影响较小。这些结果表明,针对cyclin A2的siRNAs可能成为未来抗肿瘤治疗中一种潜在的抗增殖工具。
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