Activation of distinct antiviral T-cell immunity: A comparison of bi- and trispecific T-cell engager antibodies with a chimeric antigen receptor targeting HBV envelope proteins

Bilge Debelec-Butuner; Oliver Quitt; Sophia Schreiber; Frank Momburg; Karin Wisskirchen; Ulrike Protzer

doi:10.3389/fimmu.2022.1029214

Activation of distinct antiviral T-cell immunity: A comparison of bi- and trispecific T-cell engager antibodies with a chimeric antigen receptor targeting HBV envelope proteins

Front Immunol. 2022 Nov 3:13:1029214. doi: 10.3389/fimmu.2022.1029214. eCollection 2022.

Authors

Bilge Debelec-Butuner^{1

2}, Oliver Quitt¹, Sophia Schreiber¹, Frank Momburg³, Karin Wisskirchen^{1

4}, Ulrike Protzer^{1

4}

Affiliations

¹ Institute of Virology, School of Medicine, Technical University of Munich/Helmholtz Centre Munich, Munich, Germany.
² Department of Pharmaceutical Biotechnology, Faculty of Pharmacy, Ege University, Izmir, Turkey.
³ Antigen Presentation and T/NK Cell Activation Group, Clinical Cooperation Unit Applied Tumor Immunity, German Cancer Research Centre, Heidelberg, Germany.
⁴ German Centre for Infection Research (DZIF), Munich partner site, Munich, Germany.

Abstract

Despite the availability of an effective prophylactic vaccine, 820,000 people die annually of hepatitis B virus (HBV)-related liver disease according to WHO. Since current antiviral therapies do not provide a curative treatment for the 296 million HBV carriers around the globe, novel strategies to cure HBV are urgently needed. A promising approach is the redirection of T cells towards HBV-infected hepatocytes employing chimeric antigen receptors or T-cell engager antibodies. We recently described the effective redirection of T cells employing a second-generation chimeric antigen receptor directed against the envelope protein of hepatitis B virus on the surface of infected cells (S-CAR) as well as bispecific antibodies that engage CD3 or CD28 on T cells employing the identical HBV envelope protein (HBVenv) binder. In this study, we added a trispecific antibody comprising all three moieties to the tool-box. Cytotoxic and non-cytolytic antiviral activities of these bi- and trispecific T-cell engager antibodies were assessed in co-cultures of human PBMC with HBV-positive hepatoma cells, and compared to that of S-CAR-grafted T cells. Activation of T cells via the S-CAR or by either a combination of the CD3- and CD28-targeting bispecific antibodies or the trispecific antibody allowed for specific elimination of HBV-positive target cells. While S-CAR-grafted effector T cells displayed faster killing kinetics, combinatory treatment with the bispecific antibodies or single treatment with the trispecific antibody was associated with a more pronounced cytokine release. Clearance of viral antigens and elimination of the HBV persistence form, the covalently closed circular (ccc) DNA, through cytolytic as well as cytokine-mediated activity was observed in all three settings with the combination of bispecific antibodies showing the strongest non-cytolytic, cytokine-mediated antiviral effect. Taken together, we demonstrate that bi- and trispecific T-cell engager antibodies can serve as a potent, off-the-shelf alternative to S-CAR-grafted T cells to cure HBV.

Keywords: HBV cure; T-cell engager antibody; adoptive T-cell therapy; chimeric antigen receptor; chronic hepatitis B; drug development; immunotherapy.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Antibodies, Bispecific*
Antiviral Agents
CD28 Antigens / genetics
Cytokines / genetics
DNA, Circular
Hepatitis B virus
Humans
Leukocytes, Mononuclear
Receptors, Chimeric Antigen* / genetics
T-Lymphocytes
Viral Envelope Proteins / genetics

Substances

Receptors, Chimeric Antigen
Antiviral Agents
Viral Envelope Proteins
Antibodies, Bispecific
CD28 Antigens
DNA, Circular
Cytokines