We asked how the far lower 2D affinity of the gp209–2M:HLA-A2 int

We asked how the far lower 2D affinity of the gp209–2M:HLA-A2 interaction with hCD8,

compared to interactions with the TCRs (except for W2C8), could explain the dependence of the T-cell responses on hCD8. We recently showed that mCD8 cooperates with TCR to synergistically increase the dual-receptor binding to pMHC [34]. To test whether hCD8 plays a similar Palbociclib research buy role, we used the micropipette to assay contact time-dependent adhesion frequency of RBCs bearing gp209–2M:HLA-A2 to hybridoma cells coexpressing TCR and CD8. For each of the five TCRs with a higher affinity for gp209–2M:HLA-A2 than CD8, the Pa versus tc curve followed a two-stage kinetics, exhibiting a low and a high plateau with a transition at ∼1 s in between (Supporting Information Fig. 5A–E). These characteristic binding curves are similar to those recently observed in the mouse OT1 and F5 TCRs interacting with their respective

agonist ligands [34]. To reveal the respective and the combined contributions of TCR and CD8 to each stage of the binding curve, we calculated the normalized adhesion bonds /mpMHC (Eq. (2), see Materials and methods). For the case of single-receptor interaction, the equilibrium level of /mpMHC equals the effective 2D affinity AcKa times the receptor density, mTCR or mCD8 (cf. Eq. (1) in Materials and methods). Erlotinib molecular weight For the dual-receptor case, /mpMHC provides a metric for the binding propensity that includes contributions from the TCR–pMHC and pMHC–CD8 bimolecular interactions as well as the TCR–pMHC–CD8 trimolecular interaction [34]. We plotted the contact time-dependent /mpMHC of the dual-receptor interaction (using the data from Supporting Information Fig. 5A–F) in the same graph with those of the two single-receptor interactions (using the data from Fig. 3A and B, and Supporting Information Fig. 2A–E) for each of the six TCRs (Fig. 5). In the first Farnesyltransferase five panels, the two orders of magnitude higher pMHC affinities for the TCRs than CD8

(Fig. 3C) translate to much higher /mpMHC curves for the TCRs than CD8 (Fig. 5A–E, compare circles with triangles), despite the compensation by the significantly higher CD8 densities mCD8 than the TCR densities mTCR (Fig. 1B). Remarkably, the first stage of the dual-receptor curve matches that of the TCR-only curve for each of the first five panels (Fig. 5A–E). Thus, when the hybridoma cells and RBCs make short contacts, there is little contribution to adhesion from the CD8 either by itself or in cooperation with these TCRs. This is further supported by the fact that affinities calculated from the first stage Pa (assuming no CD8 contribution) agree with the TCR–pMHC affinities measured using CD8− cell lines for five of the six TCRs with higher affinities for pMHC than CD8 (Supporting Information Fig. 5G).

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