pIRES-p16ink4a-hRb1载体的构建及其对骨肉瘤细胞周期的调控

目的应用内部核糖体插入位点(IRES)序列构建单启动子双顺反子穿梭载体pIRES-p16ink4a-hRb1并鉴定,观察其导入骨肉瘤细胞后对细胞周期的调控。方法利用基因工程技术,将p16ink4a与hRb1全长cDNA编码区依次亚克隆至pIRES载体中,质粒构建通过PCR、双酶切与测序鉴定;脂质体转染至p16ink4a表达缺失、hRb1表达阳性的骨肉瘤细胞株MG63,G418筛选获得抗性克隆,通过RT-PCR和Western blot法分析外源基因表达;流式细胞术分析细胞周期特异性和细胞凋亡率,四甲基偶氮唑蓝(MTT)比色法与细胞生长曲线观察细胞增殖情况。结果成功构建出pIRES-p16ink4a-hRb1载体,外源基因在靶细胞mRNA和蛋白水平分别有独立表达。与对照组比较,双基因导入组细胞生长抑制率显著上升,细胞周期显著阻滞在G1期,且细胞凋亡率极显著升高。结论pIRES-p16ink4a-hRb1双顺反子穿梭载体的构建与真核细胞导入、目的基因表达成功,为进一步研究p16ink4a与hRb1相互关系在细胞周期调控中的作用奠定了基础。

Effect of Exogenous p16ink4a and hRb1 Genes on Cell Cycle Regulation of Osteosarcoma Cell

To study the effect on regulation of cell cycle of osteosarcoma cell line MG63 tranceduced with exogenous p16ink4a and hRbl genes, pIRES-p16ink4a-hRb1, pIRES-p16ink4a and pIREShRbl plasmids were constructed by gene recombination technology. The recombinant plasmid was transferred into osteosarcoma cell line MG63 by metafectene, and the resistant clones were selected by G418 selective medium, mRNA and protein expression of osteosarcoma cell line were assayed by RT-PCR and Western-Blot respectively. Cell cycle and apoptosis were analyzed by subG1 flow cytometric. Cell proliferation was tested by MTT. In the genome of these transfected target cells, the expression of p16ink4a and hRb1 mRNA and protein were detected respectively in vitro. It was demonstrated with subG1 flow cytometric analysis and MTT method that p16ink4a and hRbl genes cooperation more significantly inhibited cell growth and induced a more marked G1 arrest and apoptosis than p16ink4a/hRb1 alone （P〈0.01）. Coexpression of exogenous p16ink4a with hRbl broke the regulatory feedback loop of p16ink4a-cyclinD1/CDK-hRbl and played a more significant role in inhibiting cell growth as well as inducing cell apoptosis than p16ink4a or hRbl did alone in vitro.

宣钢用SiC替代硅铁合金化冶炼HRB400EZT1钢的试验

宣钢一钢轧厂为降低吨钢生产成本、提高钢材的力学性能、改善钢水质量,调整了低合金钢合金料优质廉价碳化硅的用量,替代成本较高的硅铁和部分增碳剂使用量。在炼钢作业区110 t转炉3#炉冶炼HRB400EZT1钢进行跟踪研究,结果表明:铸坯成分稳定可控,吨钢成本可降低0.88元/t,钢材的力学性能得到改善。新合金化方案完全可以取代传统方案,获得了良好的经济效益。