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作 者:于英妮[1] 陆建华[1] 施冲[1] 曾因明[2]
机构地区:[1]广州军区广州总医院麻醉科,510010 [2]徐州医学院江苏省麻醉学重点实验室&江苏省麻醉与镇痛应用技术重点实验室
出 处:《国际麻醉学与复苏杂志》2011年第5期554-557,共4页International Journal of Anesthesiology and Resuscitation
基 金:基金项目:广东省自然科学基金面上项目(07000059);广州市科技计划项目(2010Y1-C301);广东省科技计划项目(20108031600123)
摘 要:目的探讨离体条件下水溶性纳米凝脂聚合物(water-soluble lipopolymer,WSLP)运载小干涉RNA(small interference RNA,siRNA)沉默N-甲基-天冬氨酸受体1(N-methyl—D-aspartate receptor 1,NMDAR1)基因的可行性,为在体条件下研究WSLP运载siRNA沉默NMDAR1治疗慢性疼痛等疾病打下基础。方法先合成WSLP并与NMDAR1siRNA连接成WSLP/siRNA复合物,观察其在血清中的稳定性及其对PC12细胞的毒性;然后将PC12细胞通过随机数字表法分为阴性转染组(单纯siRNA转染PC12细胞)、对照转染组(WSLP/乱序siRNA复合物转染PC12细胞)及WSLP转染组(WSLP/siRNA转染PC12细胞),通过实时-聚合酶链反应(real time polymerase chain reaction,RT-PCR)和免疫蛋白印迹法(western-blot)检测各组NMDAR1转录水平及蛋白水平基因表达的变化。结果WSLP/NMDAR1/siRNA在血清中的稳定性高,对PC12细胞几乎无毒性。与阴性转染组(0.69±0.18、4.36±1.02)相比,WSLP转染组(0.35±0.21、1.96±0.48)转录水平NMDAR1的基因表达降低50%,蛋白表达水平降低55%,差异均有统计学意义(P〈0.01),阴性转染组和对照转染组(0.64±0.13、4.32±1.09)之间的基因表达水平差异无统计学意义。结论离体条件下WSLP可有效运载siRNA沉默NMDAR1基因的表达。Objective To examine the potential application of a non-viral genecarrier, water soluble lipopolymer (WSLP) for delivering siRNA targeting N-methyl-D-aspartate receptor 1 (NMDAR1) in vitro. Methods WSLP was complexed with siRNA designed to inhibit NR1 expression. Following serum stability and cytotoxicity observation, WSLP/siRNA (scrambled siRNA as a control ) complexes were transfected in PC12 cells and then siRNA delivery efficiency of the complexes was evaluated by gene expression level assay using reverse transcriptive polymerase chain reaction (RT-PCR) and western-blot technique. Results WSLP protected siRNAs from enzymatic degradation in serum conditioned media, and the complexes of WSLP/siRNA had little cytotoxicity to cultured PC12 cell. NMDARI expression of PC12 cell was efficiently inhibited by WSLP/siRNA complexes, while complexes of WSLP with scrambled siRNA (0.64±0.13,4.32 ±1.09) did not show this inhibitory effect compared to unmodified siRNA (0.69±0.18,4.36±1.02) neither by transcriptional level nor protein level. WSLP/siRNA complexes reduced NR1 transcriptional level by 50% (0.35±0.21)and protein level by 55% (1.96±0.48) when compared to unmodified siRNA. Conclusion Our data suggest that Water soluble lipopolymer can deliver siRNA targeting NMDA receptor 1 in vitro efficiently and safely.
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