Mobilizing subdominant HIV-specific CTLS as a novel vaccine strategy

Margaret Christina Costanzo, University of Texas at El Paso

Abstract

To overcome the extreme antigenic diversity of HIV, there is increasing interest in developing vaccines that target CD8 T cell responses to conserved regions of the viral proteome. Understanding the immunogenic potential of these domains is therefore critical for the success of this vaccine strategy. CD8 T cell responses to conserved domains restricted by the "neutral" and highly prevalent HLA-A2 allele have not been extensively characterized. Here we describe a novel essentially invariant 10-mer epitope in HIV Gag (p24 14-23, RTLNAWVKVV (RV10)) in that it is expressed by the majority HIV isolates from all clades. Here we examined the character of the CD8 T cell response to this subdominant epitope in healthy volunteers and in HIV-infected individuals. RV10 was identified with in vitro immunized CD8 T cells from eight seronegative HLA-A*0201 (A*02) carriers. In brief, CD8 T cells purified by immunobeads were primed with autologous dendritic cells (DCs) transduced by a lentiviral vector to express Gag. Antigen-specific T cells were further expanded by three weekly re-stimulations with autologous monocytes pulsed with 123 15-mer overlapping peptides (OLPs) spanning across the entire Gag protein. To analyze the character of the CD8 T cell responses to RV10, TV9 and RV9, parallel cultures were generated from four healthy HLA-A*02 carriers. All cultures were stable with distinct populations of tetramer-binding cells. RV10- and TV9-specific T cells were consistently cross-reactive as measured by functional assays such as cytotoxicity and polychromatic flow cytometry. In contrast, they were less reactive to RV9. On the other hand, RV9-specific T cell cultures recognized the cognate peptide efficiently but were minimally cross-reactive to the other two peptides. Interesting to note, the three epitopes sharing the same 8-mer antigenic core display two distinct patterns of reactivities. To show that the three peptides are naturally processed and presented by MHCI molecules of infected cells, CD8 T cells were primed with autologous transduced DCs and re-stimulated with autologous transduced B cells expressing Gag. Tetramer-binding RV10-, TV9- and RV9-specific CD8 T cells were found in cultures from four of four donors, thereby indicating that these reactivities were immunized by epitopic determinants naturally processed and presented by both APCs. Alanine scanning mutagenesis revealed that substitution of asparagine (N) (position 4 of RV10 and position 3 of TV9) was associated with the most precipitous decline in recognition by RV10- and TV9-T cells, respectively. Moreover, recognition by RV10-specific T cells appeared to be more dependent on tryphtophan in position 6 than their TV9 counterparts. Of note, alanine substitutions at all positions of both peptides did not significantly reduce binding to HLA-A*02. In some instances, binding was somewhat increased. In summary, the arginine residues in these peptides appear to serve as a key TCR contact site, thereby accounting for reciprocal cross-recognition. RV10-specific T cells appeared to recognize the phenylalanine residue as well. This provides compelling albeit indirect evidence that RV10 is a distinct epitope. Here we have analyzed in detail the character of CD8 T cell responses to a set of three nested HLA-A*0201 epitopes that share a core 8-mer antigenic determinant in common. This finding has implications in T cell-based HIV vaccine design for the one of the most common HLA allele worldwide. Specifically, our data suggest a new mechanism of immunological escape ("CTL escape") by this highly variant virus. The addition of an arginine to the TV9 sequence, a seemingly useful HLA-A*02 epitope, results in immune interference due to the simultaneous presentation of cross-reactive epitopes by the same MHCI molecule, thereby preventing a full-scale activation at priming and over the long-term maintenance of Gag-specific CD8 T cell expansion. Understanding this immunological mechanism may be of great potential importance given the multiplicity of overlapping CD8 epitopes and their tendency to cluster in various HIV protein regions. (Abstract shortened by UMI.)

Subject Area

Immunology

Recommended Citation

Costanzo, Margaret Christina, "Mobilizing subdominant HIV-specific CTLS as a novel vaccine strategy" (2012). ETD Collection for University of Texas, El Paso. AAI3512004.
https://scholarworks.utep.edu/dissertations/AAI3512004

Share

COinS