Byounghoon Hwang scite author profile

Hepatitis C virus (HCV)-encoded nonstructural protein 3 (NS3) possesses protease, NTPase, and helicase activities, which are considered essential for viral proliferation. Thus, HCV NS3 is a good putative therapeutic target protein for the development of anti-HCV agents. In this study, we isolated specific RNA aptamers to the helicase domain of HCV NS3 from a combinatorial RNA library with 40-nucleotide random sequences using in vitro selection techniques. The isolated RNAs were observed to very avidly bind the HCV helicase with an apparent K d of 990 pM in contrast to original pool RNAs with a K d of >1 µM. These RNA ligands appear to impede binding of substrate RNA to the HCV helicase and can act as potent decoys to competitively inhibit helicase activity with high efficiency compared with poly(U) or tRNA. The minimal binding domain of the ligands was determined to evaluate the structural features of the isolated RNA molecules. Interestingly, part of binding motif of the RNA aptamers consists of similar secondary structure to the 3-end of HCV negative-strand RNA. Moreover, intracellular NS3 protein can be specifically detected in situ with the RNA aptamers, indicating that the selected RNAs are very specific to the HCV NS3 helicase. Furthermore, the RNA aptamers partially inhibited RNA synthesis of HCV subgenomic replicon in Huh-7 hepatoma cell lines. These results suggest that the RNA aptamers selected in vitro could be useful not only as therapeutic and diagnostic agents of HCV infection but also as a powerful tool for the study of HCV helicase mechanism.

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Prevention of passively transferred experimental autoimmune myasthenia gravis by an in vitro selected RNA aptamer

Hwang

Han

Lee

2003

FEBS Letters

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Myasthenia gravis (MG) and its animal model, experimental autoimmune MG (EAMG), are mainly caused by autoantibodies directed against acetylcholine receptors (AChR) located in the postsynaptic muscle membrane. Previously, we isolated an RNA aptamer with 2P P-£uoropyrimidines using in vitro selection techniques that acted as an e¡ective decoy against both a rat monoclonal antibody called mAb198, which recognizes the main immunogenic region on the AChR, and a signi¢cant fraction of patient autoantibodies with MG. To investigate the therapeutic potential of the RNA, we tested the ability of the RNA aptamer to protect the receptors in vivo from mAb198. Clinical symptoms of EAMG in rats engendered by passive transfer of mAb198 were e⁄ciently inhibited by a truncated RNA aptamer that was modi¢ed with polyethylene glycol, but not by control scrambled RNA. Moreover, the loss of AChR in the animals induced by the antibody was also signi¢cantly blocked with the modi¢ed RNA aptamer. These results suggested that RNA aptamers could be applied for antigen-speci¢c treatment for autoimmune diseases including MG. ß

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Improvement of RNA Aptamer Activity against Myasthenic Autoantibodies by Extended Sequence Selection

Hwang¹,

Lee²

2002

Biochemical and Biophysical Research Communications

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