Structural basis for peptide substrate specificities of glycosyltransferase GalNAc-T2

Sai Pooja Mahajan; Yashes Srinivasan; Jason W Labonte; Matthew P DeLisa; Jeffrey J Gray

doi:10.1021/acscatal.0c04609

Structural basis for peptide substrate specificities of glycosyltransferase GalNAc-T2

ACS Catal. 2021 Mar 5;11(5):2977-2991. doi: 10.1021/acscatal.0c04609. Epub 2021 Feb 19.

Authors

Sai Pooja Mahajan¹, Yashes Srinivasan², Jason W Labonte^{1

3}, Matthew P DeLisa⁴, Jeffrey J Gray^{1

5}

Affiliations

¹ Department of Chemical and Biomolecular Engineering, Johns Hopkins University, Baltimore, Maryland 21218, United States.
² Department of Bioengineering, University of California, Los Angeles, Los Angeles, California 90095, United States.
³ Department of Chemistry, Franklin & Marshall College, Lancaster, Pennsylvania 17604, United States.
⁴ Robert Frederick Smith School of Chemical and Biomolecular Engineering, Department of Microbiology, and Nancy E. and Peter C. Meinig School of Biomedical Engineering, Biochemistry, Molecular and Cell Biology, Cornell University, Ithaca, New York 14853, United States.
⁵ Sidney Kimmel Comprehensive Cancer Center, Johns Hopkins School of Medicine, Baltimore, Maryland, United States.

Abstract

The polypeptide N-acetylgalactosaminyl transferase (GalNAc-T) enzyme family initiates O-linked mucin-type glycosylation. The family constitutes 20 isoenzymes in humans. GalNAc-Ts exhibit both redundancy and finely tuned specificity for a wide range of peptide substrates. In this work, we deciphered the sequence and structural motifs that determine the peptide substrate preferences for the GalNAc-T2 isoform. Our approach involved sampling and characterization of peptide-enzyme conformations obtained from Rosetta Monte Carlo-minimization-based flexible docking. We computationally scanned 19 amino acid residues at positions -1 and +1 of an eight-residue peptide substrate, which comprised a dataset of 361 (19x19) peptides with previously characterized experimental GalNAc-T2 glycosylation efficiencies. The calculations recapitulated experimental specificity data, successfully discriminating between glycosylatable and non-glycosylatable peptides with a probability of 96.5% (ROC-AUC score), a balanced accuracy of 85.5% and a false positive rate of 7.3%. The glycosylatable peptide substrates viz. peptides with proline, serine, threonine, and alanine at the -1 position of the peptide preferentially exhibited cognate sequon-like conformations. The preference for specific residues at the -1 position of the peptide was regulated by enzyme residues R362, K363, Q364, H365 and W331, which modulate the pocket size and specific enzyme-peptide interactions. For the +1 position of the peptide, enzyme residues K281 and K363 formed gating interactions with aromatics and glutamines at the +1 position of the peptide, leading to modes of peptide-binding sub-optimal for catalysis. Overall, our work revealed enzyme features that lead to the finely tuned specificity observed for a broad range of peptide substrates for the GalNAc-T2 enzyme. We anticipate that the key sequence and structural motifs can be extended to analyze specificities of other isoforms of the GalNAc-T family and can be used to guide design of variants with tailored specificity.

Keywords: GalNAcT; O-linked glycosylation; computational specificity prediction; enzyme specificity; glycosyltransferases.

Abstract

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