| Literature DB >> 26611395 |
Li Yang1, Ya-Juan Wang1, Hai-Jun Chen2, Li-Ping Shi1, Xian-Kun Tong1, Yang-Ming Zhang2, Gui-Feng Wang1, Wen-Long Wang2, Chun-Lan Feng1, Pei-Lan He1, Yi-Bin Xu1, Meng-Ji Lu3, Wei Tang1, Fa-Jun Nan4, Jian-Ping Zuo5.
Abstract
During the hepatitis B virus (HBV) life cycle, nucleocapsid assembly is essential for HBV replication. Both RNA reverse transcription and DNA replication occur within the HBV nucleocapsid. HBV nucleocapsid is consisted of core protein (HBcAg), whose carboxy-terminal domain (CTD) contains an Arg-rich domain (ARD). The ARD of HBcAg does contribute to the encapsidation of pregenomic RNA (pgRNA). Previously, we reported a small-molecule, NZ-4, which dramatically reduced the HBV DNA level in an in vitro cell setting. Here, we explore the possible mechanisms by which NZ-4 inhibits HBV function. As an HBV inhibitor, NZ-4 leads to the formation of genome-free capsids, including a new population of capsid that runs faster on agarose gels. NZ-4's activity was dependent on the presence of the ARD I, containing at least one positively charged amino acid. NZ-4 might provide a new option for further development of HBV therapeutics for the treatment of chronic hepatitis B.Entities:
Keywords: Anti-hepatitis B virus compound; Arg-rich domain I; Capsid formation; Faster-migrating capsid; pgRNA packaging
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Year: 2015 PMID: 26611395 DOI: 10.1016/j.antiviral.2015.11.004
Source DB: PubMed Journal: Antiviral Res ISSN: 0166-3542 Impact factor: 5.970