Stabilization of soluble, low-affinity HLA-DM/HLA-DR1 complexes by leucine zippers

Robert Busch, Achal Pashine, K Christopher Garcia, Elizabeth D Mellins

Research output: Contribution to journalArticlepeer-review

Abstract

The ectodomains of interacting membrane-bound proteins, when expressed as recombinant soluble molecules, often have low affinities for each other, hampering studies of their interaction. We reasoned that stabilization of unstable protein-protein complexes should aid our understanding of the structural and functional consequences of complex formation. Here, we have used fusion with leucine zipper (LZ) domains to stabilize a complex formed between the class II major histocompatibility complex (MHC-II) protein, HLA-DR1 (which binds peptides for presentation to CD4+ T cells) and HLA-DM (which catalyzes peptide exchange of MHC-II molecules). To this end, the DM beta chain ectodomains were fused to acidic LZ domains (AcidP1 or Fos); similarly, the DR1 beta chain ectodomains were fused to basic LZ domains (BaseP1 or Jun). We expressed LZ-modified soluble DM or DR1 alphabeta dimers, or both, in insect cells and purified the secreted sDM-AcidP1 and sDR1-BaseP1 molecules as well as the complex. LZ modification greatly enhanced DM-catalyzed peptide binding to DR1 compared to unmodified soluble DM and DR1. We readily detected LZ-modified DM/DR complexes on native PAGE gels and by coimmunoprecipitation. Thus, fusion with artificial LZ domains can stabilize unstable protein-protein complexes for biochemical and structural studies of interactions within the complex.

Original languageEnglish
Pages (from-to)111-21
Number of pages11
JournalJournal of immunological methods
Volume263
Issue number1-2
Publication statusPublished - 1 May 2002

Keywords

  • Animals
  • Cell Line
  • Dimerization
  • Drosophila melanogaster
  • Genetic Techniques
  • HLA-D Antigens
  • HLA-DR1 Antigen
  • Peptides
  • Solubility
  • Zinc Fingers

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