4a), we also tested these alleles. CatG digested I-Ag7, but not I-Ek (Fig. 4c), indicating that the Q to E change in I-Ek influences check details the ability of CatG to cleave at that site. Published sequences suggest that HLA-DR, -DQ and -DP alleles are susceptible to CatG (http://www.ebi.ac.uk/imgt/hla/)35 and I-A, but not I-E, alleles are susceptible to CatG. The sequence
of DMβ predicted that this protein would be resistant to CatG cleavage on the fx1/fx2 loop. Insect cell-derived soluble DM (sDM) was resistant to proteolysis by CatG, at both pH 5 and pH 7, but was cleaved by the lysosomal cysteine proteases CatL and CatB at pH 5 (Fig. 4d). We concluded that CatG is capable of initiating proteolysis of many MHC II alleles (but not sDM) at a specific β chain cleavage site in vitro. Given the evidence that DM is able to preserve MHC II binding sites and is thought to rescue MHC II molecules from degradation,36,37 we hypothesized that DM/MHC II complexes might be resistant to CatG. Stable, covalent complexes of HLA-DR and DM are not available, selleck kinase inhibitor and sDR molecules in reversible complexes formed by engineering DM and HLA-DR with complementary leucine-zippers28 remain CatG susceptible (not shown). To address whether DM and CatG interaction sites might overlap, we tested the CatG susceptibility of a series of purified,
full-length mutant HLA-DR molecules, carrying substitutions that had previously been shown to disrupt DM interaction. Two mutations related to the DM interface on HLA-DR conferred some resistance to CatG (Fig. 5a). The mutation in one resistant mutant (DR βD152N) results in addition of an aberrant glycan on the DM interaction face of HLA-DR. The second resistant mutant introduces a positively charged lysine for a glutamic acid (βE187K). Although the amount of input DR was somewhat variable, this is unlikely to have confounded our results, because the resistant mutant DR molecules were not present in excessive amounts (thus the lack of inhibition was not a result of substrate inhibition),
nor in quantities too small to allow detection of β-chain degradation (as confirmed by overexposure of the blots shown). The positions of the mutations and the CatG cleavage site are indicated in Fig. 5b on the crystal Osimertinib datasheet structure of HLA-DR1. The former mutation probably sterically inhibits CatG access to its cleavage site, while the latter may introduce charge repulsion of the highly cationic CatG at a region of HLA-DR involved in CatG binding. HLA-DR molecules with mutations in other regions remained susceptible (Fig. 5a and data not shown). Together these results implicate the membrane-proximal portion of the DM interface on HLA-DR in CatG binding and suggest, but do not prove, that DM binding may protect MHC II molecules from CatG digestion.