HLA-B-ASTERISK-3501 - PEPTIDE INTERACTIONS - ROLE OF ANCHOR RESIDUES OF PEPTIDES IN THEIR BINDING TO HLA-B-ASTERISK-3501 MOLECULES

被引:0
|
作者
TAKAMIYA, Y
SCHONBACH, C
NOKIHARA, K
YAMAGUCHI, M
FERRONE, S
KANO, K
EGAWA, K
TAKIGUCHI, M
机构
[1] UNIV TOKYO, INST MED SCI, DEPT TUMOR BIOL, MINATO KU, TOKYO 108, JAPAN
[2] TOKYO UNIV AGR & TECHNOL, FUCHU, TOKYO 183, JAPAN
[3] SHIMADZU CO, DEPT BIOTECHNOL INSTRUMENTS, KYOTO, JAPAN
[4] OLYMPUS OPT CO LTD, BIOMED RES CTR, TOKYO, JAPAN
[5] NEW YORK MED COLL, DEPT MICROBIOL & IMMUNOL, VALHALLA, NY 10595 USA
关键词
ANCHOR RESIDUE; HLA-B35; MOLECULES; PEPTIDE MOTIFS; SELF-PEPTIDE;
D O I
暂无
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Two HLA-B*3501 binding self-peptides, LPFDFTPGY (37F) and LPGPKFLQY (28H), were isolated from HLA-B*3501 molecules expressed by cultured human B lymphoid cells. Both sequences were consistent with previously reported motifs of HLA-B*3501 binding peptides which carry proline at position 2 and tyrosine at position 9 as anchor residues. Direct binding of these peptides to HLA-B*3501 molecules was quantitated by flow cytometry analysis of RMA-S cells transfected with the HLA-8*3501 gene (RMA-S-B*3501). Both 37F and 28H peptides bound effectively to HLA-B*3501 molecules. Substitution of amino acids at position 2 and/or 9 of HLA-B*3501 binding peptides markedly reduced their binding to HLA-B*3501 molecules. These results indicate that two anchor residues, proline at position 2 and tyrosine at position 9 are critical in binding of peptides to HLA-B*3501 molecules. Insertion of up to four glycine residues at position 8 of the peptide 37F did not affect its binding affinity to HLA-B*3501 molecules. These results indicate that long peptides can effectively bind to HLA class I molecules provided that anchor residues are conserved.
引用
收藏
页码:255 / 261
页数:7
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