Several trinitrophenyl (TNP)-specific mouse cytotoxic T cell (CTL) clones recognize TNP-conjugated peptides in association with class I MHC molecules (‘hapten-peptide determinants’). However, cell modification with trinitrobenzene sulfonic acid (TNBS) also leads to the formation of TNP determinants covalently attached to MHC molecules (‘altered self’). To determine the importance of ‘peptide’ versus ‘altered self’ determinants, we used the mutant cell line RMA-S which expresses peptide-free (‘empty’) K^b and D^b molecules at 26°C. Additionally, we stabilized K^b molecules on RMA-S cells at 37°C using the K^b binding heptapeptide N53–59 derived from the vesicular stomatitis virus nucleoprotein. Lacking lyslne, this peptide remains unmodified by TNBS and, therefore, only allows the formation of ‘altered self’ TNP determinants on occupied Kb molecules. RMA-S targets, pretreated or untreated with N53–59, upon TNBS modification were only lysed poorly or not at all by four different TNP-specific CTL. In contrast, all of these clones efficiently lysed TNBS-treated, unmutated RMA cells, and three of them strongly reacted with RMA or RMA-S cells in the presence of tryptic TNP-BSA peptides. Moreover, the clone unreactlve for TNP-BSA peptides also recognized TNP sef-peptides extracted from TNBS-treated syngeneic spleen cells. Taken together, these data clearly show that TNP residues linked to MHC via associated peptides but not by covalent bondage represent the dominant antlgenic epitopes for class I MHC-restricted, hapten-specific T cells.