Yin Liusong, Trenh Peter, Guce Abigail, Wieczorek Marek, Lange Sascha, Sticht Jana, Jiang Wei, Bylsma Marissa, Mellins Elizabeth D, Freund Christian, Stern Lawrence J
From the Program in Immunology and Microbiology and.
Department of Pathology, University of Massachusetts Medical School, Worcester, Massachusetts 01605.
J Biol Chem. 2014 Aug 22;289(34):23449-64. doi: 10.1074/jbc.M114.585539. Epub 2014 Jul 7.
HLA-DM mediates the exchange of peptides loaded onto MHCII molecules during antigen presentation by a mechanism that remains unclear and controversial. Here, we investigated the sequence and structural determinants of HLA-DM interaction. Peptides interacting nonoptimally in the P1 pocket exhibited low MHCII binding affinity and kinetic instability and were highly susceptible to HLA-DM-mediated peptide exchange. These changes were accompanied by conformational alterations detected by surface plasmon resonance, SDS resistance assay, antibody binding assay, gel filtration, dynamic light scattering, small angle x-ray scattering, and NMR spectroscopy. Surprisingly, all of those changes could be reversed by substitution of the P9 pocket anchor residue. Moreover, MHCII mutations outside the P1 pocket and the HLA-DM interaction site increased HLA-DM susceptibility. These results indicate that a dynamic MHCII conformational determinant rather than P1 pocket occupancy is the key factor determining susceptibility to HLA-DM-mediated peptide exchange and provide a molecular mechanism for HLA-DM to efficiently target unstable MHCII-peptide complexes for editing and exchange those for more stable ones.
HLA - DM在抗原呈递过程中介导加载于MHCII分子上的肽段交换,其机制尚不清楚且存在争议。在此,我们研究了HLA - DM相互作用的序列和结构决定因素。在P1口袋中相互作用不理想的肽段表现出低MHCII结合亲和力和动力学不稳定性,并且对HLA - DM介导的肽段交换高度敏感。这些变化伴随着通过表面等离子体共振、SDS抗性测定、抗体结合测定、凝胶过滤、动态光散射、小角X射线散射和核磁共振光谱检测到的构象改变。令人惊讶的是,所有这些变化都可以通过替换P9口袋锚定残基来逆转。此外,P1口袋和HLA - DM相互作用位点之外的MHCII突变增加了对HLA - DM的敏感性。这些结果表明,动态的MHCII构象决定因素而非P1口袋占据情况是决定对HLA - DM介导的肽段交换敏感性的关键因素,并为HLA - DM有效靶向不稳定的MHCII - 肽复合物以进行编辑并将其替换为更稳定的复合物提供了分子机制。
