Abstract
Asparaginyl endopeptidases (AEPs) or legumains are Asn/Asp (Asx)-specific proteases that break peptide bonds, but also function as peptide asparaginyl ligases (PALs) that make peptide bonds. This ligase activity can be used for site-specific protein modifications in biochemical and biotechnological applications. Although AEPs are common, PALs are rare. We previously proposed ligase activity determinants (LADs) of these enzymes that could determine whether they catalyze formation or breakage of peptide bonds. LADs are key residues forming the S2 and S1′ substrate-binding pockets flanking the S1 active site. Here, we build on the LAD hypothesis with the engineering of ligases from proteases by mutating the S2 and S1′ pockets of VcAEP, an AEP from Viola canadensis. Wild type VcAEP yields <5% cyclic product from a linear substrate at pH 6.5, whereas the single mutants VcAEP-V238A (Vc1a) and VcAEP-Y168A (Vc1b) targeting the S2 and S1′ substrate-binding pockets yielded 34 and 61% cyclic products, respectively. The double mutant VcAEP-V238A/Y168A (Vc1c) targeting both the S2 and S1′ substrate-binding pockets yielded >90% cyclic products. Vc1c had cyclization efficiency of 917,759 M−1s−1, which is one of the fastest rates for ligases yet reported. Vc1c is useful for protein engineering applications, including labeling of DARPins and cell surface MCF-7, as well as producing cyclic protein sfGFP. Together, our work validates the importance of LADs for AEP ligase activity and provides valuable tools for site-specific modification of proteins and biologics.
Highlights
Asparaginyl endopeptidases (AEP), known as legumain and vacuolar processing enzymes (VPE), belong to the C13 family of cysteine proteases, which break peptide bonds after Asn/Asp (Asx) residues (Abe et al, 1993; Bottari et al, 1996; Shimada et al, 2003)
We showed the importance of LAD2 for controlling ligase activity of AEPs by generating several AEP mutants derived from Viola yedoensis (VyPAL3-Y175G) and Viola canadensis (VcAEP-Y168A) (Hemu et al, 2019)
We successfully engineer an AEP from Viola canadensis to an AEP-type ligase or peptide asparaginyl ligases (PALs) by mutating the residues that reside in the substrate-binding pockets flanking the S1 active site
Summary
Asparaginyl endopeptidases (AEP), known as legumain and vacuolar processing enzymes (VPE), belong to the C13 family of cysteine proteases, which break peptide bonds after Asn/Asp (Asx) residues (Abe et al, 1993; Bottari et al, 1996; Shimada et al, 2003). AEPs are well studied in plants and are multifaceted enzymes that display three distinct enzymatic functions: proteolysis, splicing, and ligation. AEPs were discovered as endopeptidases in the early 1990s, but were shown to be splicing enzymes that posttranslationally modify the circularly permutated lectin concanavalin A (Min and Jones 1994; Nonis et al, 2021). AEPs play important roles in processing seed storage proteins to release nutrients and bioactive peptides, forming seed coats, regulating programmed cell death, and generating host-defense antimicrobial and anti-fungal peptides (Hara-Nishimura, Inoue and Nishimura 1991; Saska et al, 2007; Hatsugai et al, 2015; Dall and Brandstetter 2016; Loo et al, 2016; Yamada et al, 2020)
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