[19-21] Hence, the tripartite extracellular interaction between TCR, pMHCI and CD8 (Fig. 1) has important consequences in terms of intracellular signalling.[22] Although it is now generally accepted that CD8 enhances antigen sensitivity, recent studies have shown that certain
CD8+ T-cell responses can occur independently of the CD8 co-receptor.[23] This review will cover newly reported molecular aspects of the pMHCI–CD8 interaction and the role of the co-receptor during CD8+ T-cell antigen surveillance. The CD8 co-receptor binds to a largely invariant region of MHCI that is spatially distinct from the TCR binding platform, allowing the potential for tripartite (TCR–pMHCI–CD8) complex formation (Fig. 1). In an analogous fashion to the TCR, the soluble domain of CD8 contains a number of flexible complementarity-determining EX 527 concentration region-like (CDR) loops that are involved in MHCI binding. The interaction
between the CDR-like loops of human CD8αα (residues 51–55) and a finger-like loop in the α3 domain of HLA-A*0201 (residues 223–229) forms the main contact zone of the complex. The CDR-like loops of CD8αα ‘clamp’ onto this flexible finger-like loop asymmetrically, with each molecule in the dimer contributing differently to the overall binding (Fig. 2c). Additionally, CD8αα contacts the α2 and β2m domains of HLA-A*0201, compounding the overall stability of the complex.[24, 25] These findings have been confirmed recently by another study that reported selleck inhibitor the co-crystal structure of CD8αα in complex with HLA-A*2402.[26] In this structure, CD8αα bound primarily to the flexible α3 domain of HLA-A*2402 in a virtually identical conformation
to that observed with HLA-A*0201.[26] Although Interleukin-3 receptor murine CD8αα bound to H2-Kb in a similar fashion compared with the human HLA-A*0201-CD8αα complex,[27] there were some key differences in fine specificity between these two interactions. For example, in the murine system, more contacts were made between CD8 and the MHCI α3 domain, fewer contacts existed between CD8 and the MHCI α2 domain, and a number of unique bonds were formed at the interface between CD8 and β2m. These differences probably explain the higher binding affinity of murine CD8 compared with human CD8 for their corresponding species-specific MHCIs.[15] Until recently, the orientation of the CD8αβ heterodimer in complex with pMHCI remained speculative.[28] The atomic structure of murine CD8αβ in complex with H-2Dd[29] revealed that the binding mode of the CD8αβ heterodimer was largely homologous to that of the CD8αα homodimer.[24, 27] Accordingly, the CDR-like loops of CD8αβ bound predominantly to the conserved finger-like loop in the H-2Dd α3 domain (Fig. 2d). Moreover, CD8αβ adopted a single orientation in the H-2Dd–CD8αβ co-complex, with the β-chain in the equivalent position to the CD8 α1-chain in the pMHCI–CD8αα complex, proximal to the T-cell membrane, in opposition to the original structural conformation predicted previously[24] (Fig. 2d).