Knockdown of Virus Antigen Expression Increases Therapeutic Vaccine Efficacy in High-titer HBV Carrier Mice
Thomas Michler1,10, ∗
, Anna D. Kosinska1,10, ∗
, Julia Festag1
, Till Bunse1,10
, Jinpeng Su1
, Marc Ringelhan1,2
, Hortenzia Imhof1
, Dirk Grimm3,10
, Katja Steiger4
, Carolin Mogler4
, Mathias Heikenwalder5
, Marie-Louise Michel6
, Carlos A. Guzman7,10
, Stuart Milstein8
, Laura Sepp-Lorenzino8
, Percy Knolle9,10
, Ulrike Protzer1,10, ∗, 'Correspondence information about the author Ulrike ProtzerEmail the author Ulrike ProtzerEmail the author Ulrike Protzer
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DOI: https://doi.org/10.1053/j.gastro.2020.01.032
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Publication History
Published online: January 28, 2020Accepted: January 20, 2020Received in revised form: December 28, 2019Received: June 5, 2019
Abstract
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Background & Aims
Hepatitis B virus (HBV) infection persists because the virus-specific immune response is dysfunctional. Therapeutic vaccines might be used to end immune tolerance to the virus in patients with chronic infection, but these have not been effective in patients. In patients with chronic HBV infection, high levels of virus antigens might prevent induction of HBV-specific immune responses. We investigated whether knocking down expression levels of HBV antigens in liver might increase the efficacy of HBV vaccines in mice.
Methods
We performed studies with male C57BL / 6 mice that persistently replicate HBV (genotype D, serotype ayw) —either from a transgene or after infection with an adeno-associated virus that transferred an overlength HBV genome—and expressed HB surface antigen (HBsAg) at levels relevant to patients. Small hairpin or small interfering (si) RNAs against the common 3'-end of all HBV transcripts were used to knock-down antigen expression in mouse hepatocytes. siRNAs were chemically stabilized and conjugated to N-acetylgalactosamine to increase liver uptake. Control mice were given either entecavir or non-HBV specific siRNAs and vaccine components. Eight to twelve weeks later, mice were immunized twice with a mixture of adjuvanted HBV S and core antigen, followed by a modified vaccinia virus Ankara vector to induce HBV -specific B- and T-cell responses. Serum and liver samples were collected and analyzed for HBV-specific immune responses, liver damage, and viral parameters.
Results
In both models of HBV infection, mice that express hepatocyte-specific small hairpin RNAs or that were given subcutaneous injections of siRNAs had reduced levels of HBV antigens, HBV replication, and viremia (1–3 log10 reduction), compared to mice given control RNAs . Vaccination induced production of HBV-neutralizing antibodies, and increased numbers and functionality of HBV-specific, CD8 + T-cells in mice with low, but not in mice with high levels of HBV antigen. Mice with initially high titers of HBV and knockdown of HBV antigen expression, but not mice with reduced viremia following administration of entecavir, developed polyfunctional, HBV-specific CD8 + T cells and HBV was eliminated.
Conclusions
In mice with high levels of HBV replication, knockdown of HBV antigen expression along with a therapeutic vaccination strategy, but not knockdown alone, increased numbers of effector T cells and eliminated the virus. These findings indicate that high titers of virus antigens reduce the efficacy of therapeutic vaccination. Anti-HBV siRNAs and therapeutic vaccines are each being tested in clinical trials—their combination might cure chronic HBV infection.
Keywords:
Viral hepatitis, immunization, siRNA, immunotherapy作者: StephenW 时间: 2020-2-18 17:08