Phosphorylation of the Core Protein of Hepatitis B Virus by a 46-Kilodalton Serine Kinase

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J Virol, May 1998, p. 3796-3803, Vol. 72, No. 5
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Phosphorylation of the Core Protein of Hepatitis B Virus by a 46-Kilodalton Serine Kinase

Jyh-Hwa Kau and Ling-Pai Ting^*

Institute of Microbiology and Immunology, School of Life Science, National Yang-Ming University, Shih-Pai, Taipei 11221, Taiwan, Republic of China

Received 16 September 1997/Accepted 2 February 1998

Core protein is the major component of the core particle (nucleocapsid) of human hepatitis B virus. Core particles and coreproteins are involved in a number of important functions in thereplication cycle of the virus, including RNA packaging, DNA synthesis,and recognition of viral envelope proteins. Core protein is aphosphoprotein with most, if not all, of the phosphorylation onC-terminal serine residues. In this study, we identified a serinekinase activity from the ribosome-associated protein fractionof cytoplasm that could specifically bind and phosphorylate theC-terminal portion of recombinant core protein. This kinase isreferred to as core-associated kinase (CAK). CAK could be inhibitedby the kinase inhibitors heparin and manganese ions but not byspermidine, DRB, H89, or H7, indicating that CAK is distinct fromprotein kinase A and protein kinase C. CAK could be partiallypurified by heparin-Sepharose CL-6B and phosphocellulose P11 columns.By using a far-Western assay, three specific proteins, of 46,35, and 13 kDa, were shown to interact with the C-terminal partof the core protein. These three proteins were present only inthe eluted fractions that contains the CAK activity. An in-gelkinase assay showed that a 46-kDa kinase in the same fractioncould bind and phosphorylate the C-terminal part of the recombinantcore protein. These results indicate that this 46-kDa kinase ismost probably CAK. A similar 46-kDa kinase, which exhibits thesame profile of sensitivity to kinase inhibitors as that of CAK,is present in both purified intracellular core particles and extracellular42-nm virions, suggesting that CAK is a candidate for the coreparticle-associated kinase.

^* Corresponding author. Mailing address: Institute of Microbiology and Immunology, School of Life Science, National Yang-MingUniversity, Shih-Pai, Taipei 11221, Taiwan. Phone: 2-28222400.Fax: 2-28212880. E-mail: lpting{at}ym.edu.tw.

J Virol, May 1998, p. 3796-3803, Vol. 72, No. 5
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

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