Anti-HLA-E mAb 3D12 mimics MEM-E/02 in binding to HLA-B and HLA-C alleles: Web-tools validate the immunogenic epitopes of HLA-E recognized by the antibodies

被引:29
作者
Ravindranath, Mepur H. [1 ]
Tho Pham [1 ]
El-Awar, Nadim [2 ]
Kaneku, Hugo [1 ]
Terasaki, Paul I. [1 ]
机构
[1] Terasaki Fdn Lab, Los Angeles, CA 90064 USA
[2] One Lambda Inc, Canoga Pk, CA 91303 USA
关键词
HLA: human leukocyte antigen; Classical HLA class la (HLA-la); HLA-A; HLA-B; HLA-C; HLA-E; HLA-F; HLA-G; HLA-E-mAbs: anti-HLA-E monoclonal antibodies (mAb); mAb; 3D12; mAb MEM-E/02; Epitopes; Epitope prediction web-tools; ElliPro; Mean fluorescent index (MEI); Luminex Multiplex Flowcytometric technology; ALPHA-HELIX STABILITY; ANTIGENIC DETERMINANTS; SURFACE EXPRESSION; PROTEINS; PREDICTION; RELEASE; CHAINS;
D O I
10.1016/j.molimm.2010.09.011
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
070307 [化学生物学]; 071010 [生物化学与分子生物学];
摘要
HLA-E shares several peptide sequences with HLA-class la molecules. Therefore, anti-HLA-E antibodies that recognize the shared sequences may bind to HLA-class la alleles. This hypothesis was validated with a murine anti-HLA-E monoclonal antibody (mAb) MEM-E/02, which reacted with microbeads coated with several HLA-B and HLA-C antigens. In this report, the hypothesis was reexamined with another mAb 3D12, considered to be specific for HLA-E. The antibody binding is evaluated by measuring mean fluorescence index [MFI] with Luminex Multiplex Flow-Cytometric technology. The peptide-inhibition experiments are carried out with synthetic shared peptides, most prevalent to HLA-E and HLA-la alleles. The results showed that mAb 3D12 simulated MEM-E/02 in recognizing several HLA-B and HLA-C antigens. Both 3D12 and MEM-E/02 did not bind to HLA-A, HLA-F and HLA-G molecules. As observed with MEM-E/02, binding of 3D12 to HLA-E is inhibited by the peptides sequences (115)QFAYDGKDY(123) and (137)DTAAQI(142). Decrease in binding of mAb 3D12 to HLA class la, after heat treatment of antigen coated microbeads, supports the contention that the epitope may be located at the outside of the "thermodynamically stable" alpha-helix conformations of HLA-E. Several sequence and structure-based web-tools were employed to validate the discontinuous epitopes recognized by the mAbs. The scores obtained by these web-tools distinguished the shared peptide sequences that inhibited the mAb binding to HLA-E. Furthermore, ElliPro web tool points out that both mAbs recognize the conformational discontinuous epitopes (the shared inhibitory peptide sequences) in the secondary structure of the H1A-E molecule. The study favors the contention that the domain of the shared inhibitory peptide sequences may be the most immunogenic site of HLA-E molecule. It also postulates and clarifies that amino acid substitution on or near the binding domains may account for the lack of cross reactivity of 3D12 and MEM-E/02 with HLA-A, HLA-F and HLA-G molecules. (C) 2010 Elsevier Ltd. All rights reserved.
引用
收藏
页码:423 / 430
页数:8
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