纳米粒子介导特异基因转染的实验研究  被引量：21

作　　者：李拥军[1] 管珩[1] 刘昌伟[1] 郑曰宏[1] 赵三妹[2] 王宗立[2] 杨菁[3] 宋存先[3] 

机构地区：[1]中国医学科学院中国协和医科大学北京协和医院基本外科,100730 [2]中国医学科学院基础医学研究所病理室 [3]中国医学科学院生物医学工程研究所第七研究室

出　　处：《中华医学杂志》2002年第5期341-344,共4页National Medical Journal of China

基　　金：国家自然科学基金资助(39870 196 );中国医学科学院科研重点基金资助 ( 9710 13)

摘　　要：目的　观察纳米粒子携带特异性基因转染的可行性及其效率。方法　应用聚乳酸聚乙醇酸共聚物和聚乙烯醇包载特异性反义单核细胞趋化蛋白 1基因 ,制备纳米级粒子混合物。检测其包埋率、体外释放情况及粒度。以阳离子脂质体为对照 ,利用培养的平滑肌细胞 ,应用聚合酶链反应(PCR)观察其为真核细胞传递基因的可能性 ;采用移植静脉内膜增生动物模型 ,应用RNA斑点杂交和病理形态学分析 ,观察其在体内的基因转染、表达及生物学效应。结果　制备的纳米粒子 DNA粒度为 1 50～ 30 0nm ,包埋率为 :0 .9% ,体外释放时间为 2周左右。PCR结果提示 :纳米粒子可将目的基因转移至平滑肌细胞中。体内实验显示 :纳米粒子可实现体内局部基因转染、表达 ,发挥相应的效应。Objective To evaluate the possibility and efficiency of nanoparticle as a new vector in specific gene transference. Methods Nanoparticle DNA complex was prepared with PLGA bearing antisense monocyte chemotactic protein 1 (A MCP 1), a specific expression gene, and the package efficiency, release progress in vitro, and size of the complex were determined. The nanoparticl DNA was trasnsfected into the cultured smooth muscle cells. PCR was used to evaluate the transfection of A MCP 1. Cationic lipid (lipofectamine) was used to transfect A MCP 1 as control. Forty eight hours later, DNA in the SMCs was extracted and examined by PCR. Twenty New Zealand White rabbits underwent jugular vein to artery bypass grafting procedure, of which 6 received grafts transfected with nanopaticle A MCP 1 (200 μg), 6 received grafts with cationic liposome (DOTAP) A MCP 1 (200 μg), 4 received grafts with LNCX plasmid, and 4 received grafts without transfection as control. Fourteen days after surgery grafts were harvested. The expression of A MCP 1 and its effect on MCP 1 in vein grafts were detected by dot blotting. The morphology of the grafts was investigated. Results The package efficiency, release progress in vitro , and size of the nanoparticle DNA complex thus prepared were 0.9%, 2 week, and 150 nm～300 nm respectively. Genomic DNA PCR showed that A MCP 1 gene could be successfully transfected into smooth muscle cells by nanoparticle. Two weeks later, antisense MCP 1 was expressed in the vasculat walls of the groups with transfection methods by nanaoparticle or by cationic lipid to an almost same degree. The degree of vascular hyperplasia in gene transfection groups was lower than that in control group. There was no significant difference in inhibition of intimal hyperplasia between the two groups of transfection by different vectors. Conclusion Nanoparticle acts as a vector to transfect specific gene in vitro and in vivo.

关 键 词：基因治疗 载体 纳米粒子 反义单核细胞趋化因子 血管再狭窄 基因转染 实验研究 

分 类 号：R346[医药卫生—基础医学]