CD40发夹siRNA真核表达载体构建及其对CA46细胞CD40表达的影响  被引量：5

作　　者：陈凌[1] 郑祥雄[1] 

机构地区：[1]福建医科大学附属协和医院临床免疫研究所,福建福州350001

出　　处：《细胞与分子免疫学杂志》2005年第2期163-166,共4页Chinese Journal of Cellular and Molecular Immunology

基　　金：福建省科技厅课题资助项目(No.C0310019)

摘　　要：　目的: 构建人类CD40膜蛋白siRNA的真核表达载体, 观察其对CA46细胞上CD40表达、细胞增殖能力和凋亡的影响。方法: 合成两条编码发夹siRNA序列的单链DNA,并将其克隆到pSilenCircle载体中, 构建含目的基因片段的重组质粒siCD40 /pSilenCircle。以同样的方法, 分别构建相对应的编码反义RNA及无关基因的重组质粒antiCD40 /pSilenCir cle和siFly/pSilenCircle。以上述重组质粒分别瞬时转染CA46细胞后, 用流式细胞仪检测CA46细胞上CD40的表达和细胞凋亡情况, 用MTS法(改良的MTT法)测定细胞的增殖能力。结果: ①成功地构建了两个CD40发夹siRNA的真核表达载体siCD40 /pSilenCircle、两个相对应的反义RNA真核表达载体antiCD40 /pSilenCircle和无关基因重组质粒siFly/pSilenCir cle。②与siFly/pSilenCircle转染组相比较, siCD40 /pSilenCir cle转染组和antiCD40 /pSilenCircle转染组CA46细胞上CD40的表达均明显减少, 但细胞的增殖能力和凋亡未发现明显变化。结论: 构建的两个CD40发夹siRNA的真核表达载体siCD40 /pSilenCircle, 可有效地抑制CA46细胞上CD40分子的表达, 但不影响细胞的增殖和凋亡。RNA干扰技术可望作为一种有效地调控基因功能的方法。AIM: To construct human CD40 hairpin siRNA eukaryotic expression vectors and investigate their effects on CD40 expression, proliferation and apoptosis of CA46 cells. METHODS: Two DNA oligonucleotides encoding CD40 hairpin siRNAs were synthesized, and cloned into pSilenCircle to construct recombinant plasmid siCD40/pSilenCircle that expressed hairpin siRNAs under the control of pol III U6 promoter. At the same time, antiCD40/pSilenCircle encoding the antisense CD40 RNA and siFly/pSilenCircle encoding siRNA against luciferase were constructed as control vectors. The recombinants were identified by restriction enzyme digestion analysis and sequencing. The recombinant plasmids were transfected into CA46 cells. CD40 expression on CA46 cells and apoptosis were detected by flow cytometry. The proliferation of transfected CA46 cells was detected by MTS colorimetry. RESULTS: (1)siCD40/pSilenCircle, antiCD40/pSilenCircle and siFly/pSilenCircle had been constructed successfully. (2)CD40 expressions on siCD40/pSilenCircle- and antiCD40/pSilenCircle-transfected CA46 cells were significantly reduced, as compared with that on siFly/pSilenCircle-transfected CA46 cells (P<0.01 and P<0.05, respectively). Both hairpin siRNAs and antisense RNA had no influence on the proliferation and apoptosis of CA46 cells. CONCLUSION: Constructed siCD40/pSilenCircle and antiCD40/pSilenCircle can significantly inhibit CD40 expression, but have no significant influence on the proliferation and apoptosis of CA46 cells.

关 键 词：RNAI SIRNA CD40 载体构建 CA46细胞 

分 类 号：R392.12[医药卫生—免疫学]