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作 者:李宏文[1] 毛青[1] 李奇芬[1] 王升启[1] 朱宝珍 郑红[1] 丁健[1]
机构地区:[1]第三军医大学西南医院全军传染病中,重庆400038
出 处:《中华肝脏病杂志》1999年第1期13-14,共2页Chinese Journal of Hepatology
基 金:国家自然科学基金资助!39570166
摘 要:在H-1δ9细胞中观察反义寡核苷酸(ASODN)及其硫代修饰物(S-ASODN)对丁型肝炎病毒(HDV)基因复制与表达的抑制作用。方法在分子水平证实互补于HDV基因链核酶自裂位点和Steml区的ASODN可抑制核酶自裂的基础上,进一步台成针对该区684-698位核苷酸的15聚ASODN及S-ASODN,在培养的HIδ细胞中加人不同寡核苷酸,分别采用ELISA和斑点杂交法检测上清中HDAg及细胞中的HDVcDNA。结果加人终浓度为6μmol/L的S-ASODN后24hH1δ9细胞中HDVRNA复制及HDAg分泌均受抑制,抑制率分别为845%和76.14%。S-ASODN的终浓度为2、4、6μmol/L时,其抑制作用呈剂量依赖关系。在同等剂量时,ASODN与S-ASODN抑制作用相近。结论提示所用ASODN及S-ASODN均能有效抑制转基因细胞中HDV基因的复制与表达,为进一步在动物体内研究S-ASODN抗HDV的作用提供了实验依据。Objective To Study inhibitory effect of an antisense oligodeoxynucleotide (ASODN) andits phosphorothioate (S-ASODN) on replication and expression of HDV in Hlδ9 cell. Methods in previousstudies, it was proved that the ASODNs which are complementary to genomic HDV ribozyme selfcleavage site and stem I regions can inhibit availably grnomic HDV ribozyme activity. In the presentstudy, a 15-iner ASODN and S-ASODS which are complementary to this region (nucleotide 684-698)were added to medium of cultured H169 cell. HDAg and HDV cDNA were detected by ELISA and Dotblot hybridization. Besults Twenty-fourrth hour aft6r 6pmol/L ASODN and S-ASODN were added, boththe secreting amount of HDAg in the supernatant and HDV RNA were inhibited. The inhibiting rateswere 76.14% and 84.50% respectively. When the concentration of S-ASODN was 2, 4. 6pmol/L, theinhibiting rate showed the feature of dosage dependence. Inhibitory effect of ASODN and S-ASODN weresimilar in the same dosage. Conclusion The results snarest that ASODN and S-ASODN can availablyinhibit replication and expression of HDV in H189 cell.
分 类 号:R512.630.5[医药卫生—内科学]
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