Enhanced in Vitro Potency and in Vivo Immunogenicity of a CTL Epitope from Hepatitis C Virus Core Protein Following Amino Acid Replacement at Secondary HLA-A2.1 Binding Positions

Overview

Journal J Clin Invest

Specialty General Medicine

Date 1998 Sep 17

PMID 9739058

Citations 24

Authors

P Sarobe

C D Pendleton

T Akatsuka

D Lau

V H Engelhard

S M Feinstone

J A Berzofsky

Affiliations

Soon will be listed here.

Abstract

Since the natural immune response to hepatitis C virus (HCV) is often unable to clear the infection, to enhance immunogenicity we studied substituted peptides from an HCV cytotoxic T lymphocyte (CTL) epitope (C7A2) from a conserved region of the HCV core protein (DLMGYIPLV) recognized by CTL lines from HLA-A2.1(+) HCV-infected patients and HLA-A2.1 transgenic mice. HLA-A2.1 binding, human and murine CTL recognition, and in vivo immunogenicity (using mice transgenic for human HLA-A2 in lieu of immunizing humans) were analyzed to define peptides with enhanced immunogenicity. Peptides substituted at position 1 showed enhanced HLA-A2 binding affinity, but paradoxically poorer immunogenicity. A peptide with Ala substituted at position 8 (8A) showed higher HLA-A2 binding affinity and CTL recognition and was a more potent in vivo immunogen in HLA-A2-transgenic mice, inducing higher CTL responses with higher avidity against native C7A2 than induced by C7A2 itself. These results suggest that peptide 8A is a more potent in vitro antigen and in vivo immunogen than C7A2 and may be useful as a vaccine component. They provide proof of principle that the strategy of epitope enhancement can enhance immunogenicity of a CTL epitope recognized by human CTL.

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