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acity of H-2Kb complexes by NY-gp34 when compared to gp34. However, binding affinity assays using TAP-deficient cells demonstrated that while both gp33 and gp34 displayed similar binding affinities PubMed ID:http://www.ncbi.nlm.nih.gov/pubmed/22189597 to H2Kb, nitrotyrosination of peptide residue 3 significantly reduced binding affinity of NY-gp34 to H-2Kb. Furthermore, the capacity of each peptide to stabilize H-2Kb complexes was also investigated using circular dichroism by assessing the thermostability of soluble H-2Kb molecules in complex with gp34 or NY-gp34. Melting temperatures were derived from changes in ellipticity at 218 nm, corresponding to loss of secondary structure during denaturation. Our analysis demonstrates that the Tm value for H-2Kb/NY-gp34 was nearly 10uC lower than for H-2Kb/gp34, reflecting the significantly reduced capacity of NY-gp34 to stabilize H-2Kb complexes. Similar very significant shifts in thermal stability were also obtained for the two MHC class I complexes upon analyzing their stability with differential scanning fluorimetry Interestingly, while the H-2Kb/NY-gp33-specific CD8+ T cell hybridoma 24H1 recognized H-2Kb+ target cells coated with both NY-gp33 and NY-gp34, it did not recognize H-2Kb/gp34 MHC complexes. Furthermore, it should also be noted that 24H1 T cells recognized H-2Kb/NY-gp34 to a higher level when compared to H-2Kb/NY-gp33. The relatively lower recognition of H-2Kb/NYgp33 by 24H1 could be explained by the protrusion of the side MHC-I-Restricted Nitrotyrosinated Neoantigen Y116. C. A novel hydrogen bond and a long ionic range interaction are formed between p3NY and the H-2Kb residues Q114 and Y116, respectively. While two hydrogen bond interactions are maintained between p3NY and R155, all interactions are lost with E152. doi:10.1371/journal.pone.0032805.g003 . The melting temperatures Tm corresponding to the mid-point of the sharp transition from folded to unfolded state were 54.460.1 and 44.560.2 for H-2Kb/gp34 and H-2Kb/NY-gp34. These significant differences in stabilization capacity were at first surprising when considering that additional hydrogen bonds and long ionic interactions are formed between NY-gp34 and H-2Kb when compared to H-2Kb/gp34. However, further comparative analysis of the two crystal structures provided an explanation to these unexpected results. In H-2Kb/NY-gp34, the side-chain of the nitrotyrosine p3NY projects within the D-pocket of H-2Kb, resulting in structural overpacking and a `strained’ overall conformation of the MHC complex. Although this has not, to our knowledge, yet been reported for MHC class I molecules, strained conformations are relatively common and have been described for several proteins including e.g. native serine protease inhibitors and spectrin SH3 core-domains. Induction of strained conformations is also important within several processes including catalysis in thymidylate synthase and nuclear transport of exportins. Proteins with strained `spring-loaded’ conformations are usually intrinsically unstable. For example, the release of the course of the strained conformation in circularly permutated barnases BMS-833923 chemical information resulted in a 20uC shift in melting temperature or in a 25-fold increase in stability for mutated serpins. In the crystal structure of the H-2Kb/NY-gp34 complex, introduction of the side chain of p3NY resulted in close contacts between the nitrotyrosinated peptide and several H-2Kb residues, forcing them away from the relaxed low-energy conformation observed in H2Kb/gp34 in order to accommod

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Author: PDGFR inhibitor