Mutational Analysis Reveals a Complex Interplay of Peptide Binding and Multiple Biological Features of HLA-B27

Galocha, Begoña; Castro, José A. Łópez de

doi:10.1074/jbc.m110.149906

Cited by 13 publications

(10 citation statements)

References 66 publications

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“…Presumably, this mechanism might largely bypass tapasinmediated peptide editing, leading to fast folding, albeit with a suboptimal peptide cargo. Indeed, B*27:06, B*27:07, B*27:09, and B*1403 did not misfold significantly in the ER (30,35). The lower stability of B*27:04 in WE-I is not obviously due to altered hydrophobicity of its peptide binding site, because the molecule itself is not altered; rather, presumably, it is due to the inability of the ERAP1 variant to generate an optimal peptide repertoire.…”

Section: Discussionmentioning

confidence: 87%

“…Only one experiment could be performed with JSL. The data concerning C1R04, except for one additional experiment included here, were reported previously (35) and are shown here only for comparison.…”

Section: Discussionmentioning

confidence: 99%

“…Second, although the influence of ERAP-1 on HLA-B27 folding was not examined, the decreased molecular stability of HLA-B27 observed in WE-I indicates that certain ERAP1 variants containing a number of AS-protective polymorphisms generate suboptimal B27 peptidomes. We have shown previously that high thermostability is a feature of three AS-associated subtypes (B*27:02, B*27:04, and B*27:05) expressed on C1R cells that is not shared by the non-ASassociated B*27:06 and B*27:09 subtypes or the AS-associated B*27:07 and B*1403 (30,35). The thermostability of B*27:04 in WE-I was closer to that of the latter subtypes, indicating that ERAP1 polymorphism protective against AS can approach the molecular stability phenotype of an ASassociated B27 subtype to that shown by non-AS-associated ones.…”

Section: Discussionmentioning

confidence: 99%

“…6). We previously reported that B*27:04 expressed on C1R cells shows very high thermostability, a feature that was shared with two other AS-associated subtypes (B*27:02 and B*27:05) but not with the non-AS-associated B*27:06 and B*27:09 (35). An equally high thermostability of B*27:04 was observed in JSL, and it was nearly as high in KNE, but WE-I showed lower thermostability even at the 4 h chase time, which best reflects the steady state of mature HLA-B27.…”

Section: Relative Expression Of B*27:04 Ligands In Distinct Erap1mentioning

confidence: 99%

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Functional Interaction of the Ankylosing Spondylitis-associated Endoplasmic Reticulum Aminopeptidase 1 Polymorphism and HLA-B27 in Vivo

García-Medel

Sanz-Bravo

Nguyen

et al. 2012

Molecular & Cellular Proteomics

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The association of ERAP1 with ankylosing spondylitis (AS)1 among HLA-B27-positive individuals suggests that ERAP1 polymorphism may affect pathogenesis by altering peptide-dependent features of the HLA-B27 molecule. Comparisons of HLA-B*27:04-bound peptidomes from cells expressing different natural variants of ERAP1 revealed significant differences in the size, length, and amount of many ligands, as well as in HLA-B27 stability. Peptide analyses suggested that the mechanism of ERAP1/HLA-B27 interaction is a variant-dependent alteration in the balance between epitope generation and destruction determined by the susceptibility of N-terminal flanking and P1 residues to trimming. ERAP1 polymorphism associated with AS susceptibility ensured efficient peptide trimming and high HLA-B27 stability. Protective polymorphism resulted in diminished ERAP1 activity, less efficient trimming, suboptimal HLA-B27 peptidomes, and decreased molecular stability. This study demonstrates that natural ERAP1 polymorphism affects HLA-B27 antigen presentation and stability in vivo and proposes a mechanism for the interaction between these molecules in AS.

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Section: Discussionmentioning

confidence: 87%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Relative Expression Of B*27:04 Ligands In Distinct Erap1mentioning

confidence: 99%

See 2 more Smart Citations

Functional Interaction of the Ankylosing Spondylitis-associated Endoplasmic Reticulum Aminopeptidase 1 Polymorphism and HLA-B27 in Vivo

García-Medel

Sanz-Bravo

Nguyen

et al. 2012

Molecular & Cellular Proteomics

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“…The amino acid occupancy at positions 114 and/or 116 have been shown to be of crucial importance for the degree of tapasin dependence among different sets of HLA-I molecules (17,20). Different amino acid occupancy at position 59 or 134 also separates tapasin-dependent allomorphs from less tapasin-dependent ones (21,49). This indicates an important role for several specific positions in the peptide-binding groove and might explain tapasin dependency to some degree.…”

Section: Discussionmentioning

confidence: 92%

Tapasin Facilitation of Natural HLA-A and -B Allomorphs Is Strongly Influenced by Peptide Length, Depends on Stability, and Separates Closely Related Allomorphs

Geironson

Thuring

Harndahl³

et al. 2013

The Journal of Immunology

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Despite an abundance of peptides inside a cell, only a small fraction is ultimately presented by HLA-I on the cell surface. The presented peptides have HLA-I allomorph-specific motifs and are restricted in length. So far, detailed length studies have been limited to few allomorphs. Peptide–HLA-I (pHLA-I) complexes of different allomorphs are qualitatively and quantitatively influenced by tapasin to different degrees, but again, its effect has only been investigated for a small number of HLA-I allomorphs. Although both peptide length and tapasin dependence are known to be important for HLA-I peptide presentation, the relationship between them has never been studied. In this study, we used random peptide libraries from 7- to 13-mers and studied binding in the presence and absence of a recombinant truncated form of tapasin. The data show that HLA-I allomorphs are differentially affected by tapasin, different lengths of peptides generated different amounts of pHLA-I complexes, and HLA-A allomorphs are generally less restricted than HLA-B allomorphs to peptides of the classical length of 8–10 aa. We also demonstrate that tapasin facilitation varies for different peptide lengths, and that the correlation between high degree of tapasin facilitation and low stability is valid for different random peptide mixes of specific lengths. In conclusion, these data show that tapasin has specificity for the combination of peptide length and HLA-I allomorph, and suggest that tapasin promotes formation of pHLA-I complexes with high on and off rates, an important intermediary step in the HLA-I maturation process.

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Polymorphisms in the F Pocket of HLA–B27 Subtypes Strongly Affect Assembly, Chaperone Interactions, and Heavy‐Chain Misfolding

Guiliano

North

Panayoitou³

et al. 2017

Arthritis & Rheumatology

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Objective HLA–B27 is associated with the inflammatory spondyloarthritides (SpA), although subtypes HLA–B*27:06 and HLA–B*27:09 are not. These subtypes differ from the HLA–B*27:05 disease‐associated allele primarily at residues 114 and 116 of the heavy chain, part of the F pocket of the antigen‐binding groove. Dimerization of HLA–B27 during assembly has been implicated in disease onset. The purpose of this study was to investigate the factors that influence differences in dimerization between disease‐associated and non–disease‐associated HLA–B27 alleles. Methods HLA–B*27:05 and mutants resembling the HLA–B*27:06 and 09 subtypes were expressed in the rat C58 T cell line, the human CEM T cell line and its calnexin‐deficient variant CEM.NKR. Immunoprecipitation, pulse–chase experiments, flow cytometry, and immunoblotting were performed to study the assembly kinetics, heavy‐chain dimerization, and chaperone associations. Results By expressing HLA–B*27:05, 06‐like, and 09 alleles on a restrictive rat transporter associated with antigen processing background, we demonstrate that a tyrosine expressed at p116, either alone or together with an aspartic acid residue at p114, inhibited HLA–B27 dimerization and increased the assembly rate. F‐pocket residues altered the associations with chaperones of the early major histocompatibility complex class I folding pathway. Calnexin was demonstrated to participate in endoplasmic reticulum (ER) stress–mediated degradation of dimers, whereas the oxidoreductase ERp57 does not appear to influence dimerization. Conclusion Residues within the F pocket of the peptide‐binding groove, which differ between disease‐associated and non–disease‐associated HLA–B27 subtypes, can influence the assembly process and heavy‐chain dimerization, events which have been linked to the initiation of disease pathogenesis.

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Mutational Analysis Reveals a Complex Interplay of Peptide Binding and Multiple Biological Features of HLA-B27

Cited by 13 publications

References 66 publications

Functional Interaction of the Ankylosing Spondylitis-associated Endoplasmic Reticulum Aminopeptidase 1 Polymorphism and HLA-B27 in Vivo

Functional Interaction of the Ankylosing Spondylitis-associated Endoplasmic Reticulum Aminopeptidase 1 Polymorphism and HLA-B27 in Vivo

Tapasin Facilitation of Natural HLA-A and -B Allomorphs Is Strongly Influenced by Peptide Length, Depends on Stability, and Separates Closely Related Allomorphs

Polymorphisms in the F Pocket of HLA–B27 Subtypes Strongly Affect Assembly, Chaperone Interactions, and Heavy‐Chain Misfolding

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