Molecular Basis for the Interaction of the Hepatitis B Virus Core Antigen with the Surface Immunoglobulin Receptor on Naive B Cells

6533b826fe1ef96bd1283f09

RESEARCH PRODUCT

Molecular Basis for the Interaction of the Hepatitis B Virus Core Antigen with the Surface Immunoglobulin Receptor on Naive B Cells

Juris Steinbergs Juris Steinbergs Tinghua Cao Paul Pumpens David R. Milich Matti Sällberg Una Lazdina Geert Leroux-roels Mats Alheim Darrel L. Peterson

subject

CD4-Positive T-Lymphocytes Immunology Naive B cell Antigen presentation Molecular Sequence Data Immunoglobulin Variable Region Mice Transgenic medicine.disease_cause Antibodies Viral Microbiology Mice Antigen Virology medicine Animals Humans Amino Acid Sequence Receptors Immunologic Hepatitis B virus Antigen Presentation B-Lymphocytes Mice Inbred BALB C biology virus diseases Antibodies Monoclonal Virology Molecular biology Hepatitis B Core Antigens digestive system diseases Peptide Fragments Virus-Cell Interactions HBcAg HBeAg Immunoglobulin M Immunoglobulin M Insect Science biology.protein Mice Inbred CBA Immunoglobulin Light Chains Binding Sites Antibody Antibody Immunoglobulin Heavy Chains Sequence Alignment

description

ABSTRACTThe nucleocapsid of the hepatitis B virus (HBV) is composed of 180 to 240 copies of the HBV core (HBc) protein. HBc antigen (HBcAg) capsids are extremely immunogenic and can activate naive B cells by cross-linking their surface receptors. The molecular basis for the interaction between HBcAg and naive B cells is not known. The functionality of this activation was evidenced in that low concentrations of HBcAg, but not the nonparticulate homologue HBV envelope antigen (HBeAg), could prime naive B cells to produce anti-HBc in vitro with splenocytes from HBcAg- and HBeAg-specific T-cell receptor transgenic mice. The frequency of these HBcAg-binding B cells was estimated by both hybridoma techniques and flow cytometry (B7-2 induction and direct HBcAg binding) to be approximately 4 to 8% of the B cells in a naive spleen. Cloning and sequence analysis of the immunoglobulin heavy- and light-chain variable (VH and VL) domains of seven primary HBcAg-binding hybridomas revealed that six (86%) were related to the murine and human VH1 germ line gene families and one was related to the murine VH3 family. By using synthetic peptides spanning three VH1 sequences, one VH3 sequence, and one VLκV sequence, a linear motif in the framework region 1 (FR1)complementarity-determining region 1 (CDR1) junction of the VH1 sequence was identified that bound HBcAg. Interestingly, the HBcAg-binding motif was present in the VL domain of the HBcAg-binding VH3-encoded antibody. Finally, two monoclonal antibodies containing linear HBcAg-binding motifs blocked HBcAg presentation by purified naive B cells to purified HBcAg-primed CD4+T cells. Thus, the ability of HBcAg to bind and activate a high frequency of naive B cells seems to be mediated through a linear motif present in the FR1-CDR1 junction of the heavy or light chain of the B-cell surface receptor.

year	journal	country	edition	language
2001-07-01

10.1128/jvi.75.14.6367-6374.2001 https://europepmc.org/articles/PMC114359/