HLA-DM catalytically enhances peptide dissociation by sensing peptide?MHC class II interactions throughout the peptide-binding cleft

被引:8
|
作者
Reyes-Vargas, Eduardo [1 ]
Barker, Adam P. [1 ,2 ]
Zhou, Zemin [1 ]
He, Xiao [1 ]
Jensen, Peter E. [1 ,2 ]
机构
[1] Univ Utah, Dept Pathol, Sch Med, Salt Lake City, UT 84112 USA
[2] ARUP Inst Clin & Expt Pathol, Dept Pathol, ARUP Labs, Salt Lake City, UT 84108 USA
关键词
antigen presentation; antigen processing; major histocompatibility complex (MHC); peptide interaction; kinetics; fluorescence anisotropy; catalysis; Michaelis-Menten; immunogenicity; immunology; MHC PROTEIN HLA-DR1; ANTIGEN PRESENTATION; INVARIANT CHAIN; CUTTING EDGE; HYDROGEN-BONDS; DR MOLECULES; CRYSTAL-STRUCTURE; COMPLEX; SUSCEPTIBILITY; EXCHANGE;
D O I
10.1074/jbc.RA119.010645
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Human leukocyte antigen-DM (HLA-DM) is an integral component of the major histocompatibility complex class II (MHCII) antigen-processing and -presentation pathway. HLA-DM shapes the immune system by differentially catalyzing peptide exchange on MHCII molecules, thereby editing the peptide-MHCII (pMHCII) repertoire by imposing a bias on the foreign and self-derived peptide cargos that are presented on the cell surface for immune surveillance and tolerance induction by CD4(+) T cells. To better understand DM selectivity, here we developed a real-time fluorescence anisotropy assay to delineate the pMHCII intrinsic stability, DM-binding affinity, and catalytic turnover, independent kinetic parameters of HLA-DM enzymatic activity. We analyzed prominent pMHCII contacts by differentiating the kinetic parameters in pMHCII homologs, observing that peptide interactions throughout the MHCII-binding cleft influence both the rate of peptide dissociation from the DM-pMHCII catalytic complex and the binding affinity of HLA-DM for a pMHCII. We show that the intrinsic stability of a pMHCII linearly correlates with DM catalytic turnover, but is nonlinearly correlated with its binding affinity. Surprisingly, interactions at the peptides N terminus up to and including MHCII position one (P1) anchor affected the catalytic turnover, suggesting that the active DM-pMHCII catalytic complex operates on pMHCII complexes with full peptide occupancy. Furthermore, interactions at the peptide C terminus modulated DM-binding affinity, suggesting distal communication between peptide interactions with the MHCII and the DM-pMHCII binding interface. Our results imply an intimate linkage between the DM-pMHCII interface and peptide-MHCII interactions throughout the peptide-binding cleft.
引用
收藏
页码:2959 / 2973
页数:15
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