针对 HBV 核心区的发夹核糖核酸酶在体外的抗病毒活性。

J Lin, Y Song, X Kong, N Xie, X Wu, N Liu, N Wang, E Cao, Y Jin
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引用次数: 0

摘要

为了研究针对HBV核心区转录本的发夹核糖核酸酶(HpRz)的体外制备和裂解,将计算机设计的针对HBV核心基因转录本的HRz基因克隆到介于5'-顺式-Rz和3'-顺式-Rz之间的载体p1.5中。32P 标记的 HpRz 转录本证明了该载体是否适合制备发夹核糖酶。用 T7 RNA 聚合酶转录含有 HBV 核心区靶 RNA 的 32P 标记 pKC 转录本,并用 PAGE 纯化。将冷的 HpRz 转录本与 32P 标记的靶 RNA 在不同条件下孵育,变性聚丙烯酰胺凝胶电泳后进行放射性显影。结果表明,HpRz 在 37 摄氏度和 12 mmol/L MgCl2 条件下具有裂解能力,核糖酶的设计是正确的。结论是体外制备的 HpRz 具有特异性催化活性,表明 HpRz 有可能在细胞内抑制 HBV 的复制。它将来可能被开发成治疗乙型肝炎的核酸药物。
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Anti-viral activity of hairpin ribozyme directed against HBV core region in vitro.

To study the preparation and cleavage of hairpin ribozyme (HpRz) directed against the transcript of HBV core region in vitro, HRz gene designed by computer targeting the transcript of HBV core gene was cloned into the vector p1.5 between 5'-cis-Rz and 3'-cis-Rz. 32P-labeled HpRz transcript proved whether the vector fit for the preparation of hairpin ribozyme. 32P-labeled pKC transcript containing HBV core region as targets-RNA was transcribed by using T7 RNA polymerase and purified by PAGE. Cold HpRz transcript was incubated with 32P-labeled target-RNAs under different conditions and radioautographed after denaturing polyacrylamide gel electrophoresis. The results showed that HpRz had the ability of cleavage at 37 degrees C and 12 mmol/L MgCl2 and the design of ribozyme was correct. It is concluded that HpRz prepared in vitro possesses specific catalytic activity, indicating that it is possible for HpRz to intracellularly inhibit the replication of HBV. It may be developed into a nucleic acid drug in the treatment of hepatitis B in the future.

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