Molecular bases of cyclic and specific disulfide interchange between human ERO1alpha protein and protein-disulfide isomerase (PDI).

In the endoplasmic reticulum (ER) of human cells, ERO1a and protein-disulfide isomerase (PDI) constitute one of the major electron flow pathways that catalyze oxidative folding of secretory proteins. Specific and limited PDI oxidation by ERO1a is essential to avoid ER hyperoxidation. To investigate how ERO1a oxidizes PDI selectively among more than 20 ER resident PDI family member proteins, we performed docking simulations and systematic biochemical analyses. Our findings reveal that a protruding b-hairpin of ERO1a specifically interacts with the hydrophobic pocket present in the redox-inactive PDI b"-domain through the stacks between their aromatic residues, leading to preferred oxidation of the C-terminal PDI a"-domain. ERO1a associated preferentially with reduced PDI, explaining the stepwise disulfide shuttle mechanism, first from ERO1a to PDI and then from oxidized PDI to an unfolded polypeptide bound to its hydrophobic pocket. The interaction of ERO1! with ERp44, another PDI family member protein, was also analyzed. Notably, ERO1a-dependent PDI oxidation was inhibited by a hyperactive ERp44 mutant that lacks the C-terminal tail concealing the substrate-binding hydrophobic regions. The potential ability of ERp44 to inhibit ERO1a activity may suggest its physiological role in ER redox and protein homeostasis.