Anti—HBV hairpin ribozyme—mediated cleavage of target RNA in vitro

To study the preparation and cleavage activity of HpRz directed against the transcript of HBV core gene in vitro. HpRz 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 whe...

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Bibliographic Details
Published in:World journal of gastroenterology : WJG 2002-02, Vol.8 (1), p.91-94
Main Authors: Song, Yu-Hu, Lin, Ju-Sheng, Liu, Nan-Zhi, Kong, Xin-Juan, Xie, Na, Wang, Nan-Xia, Jin, You-Xin, Liang, Kuo-Huan
Format: Article
Language:English
Subjects:
Base Sequence
Enzyme Activation
Genetic Therapy
Hepatitis B - therapy
Hepatitis B - virology
Hepatitis B Core Antigens - genetics
Hepatitis B virus - genetics
Humans
In Vitro Techniques
Kinetics
Molecular Sequence Data
Plasmids
RNA, Catalytic - metabolism
RNA, Viral - metabolism
RNA分裂
Transcription, Genetic
Viral Liver Diseases
乙型肝炎
抗病毒机制
靶细胞
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Summary:To study the preparation and cleavage activity of HpRz directed against the transcript of HBV core gene in vitro. HpRz 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 in vitro. 32p-labeled pKC transcript containing HBV core region as target-RNA was transcribed using T7 RNA polymerase and purified by denaturing PAGE. Cold HpRz transcript was incubated with 32p-labeled target-RNAs under different conditions and radio autographed after denaturing polyacrylamide gel electrophoresis. HpRz has the specific ability of cleavage of target RNA at 37 degrees and 12 mM MgCl2. Km=26.31 nmol/L, Kcat=0.18/min. These results revealed that the design of HpRz was correct. HpRz prepared in this study possesses specific catalytic activity from the identification of cleavage activity. These results indicate that hairpin ribozyme may intracellularly inhibit the replication of HBV, therefore it may become a novel potent weapon for the treatment of hepatitis B.
ISSN:1007-9327
2219-2840
DOI:10.3748/wjg.v8.i1.91