An Enzymatic Toolkit for Selective Proteolysis, Detection, and Visualization of Mucin-Domain Glycoproteins

18 June 2020, Version 1
This content is a preprint and has not undergone peer review at the time of posting.

Abstract

Densely O-glycosylated mucin domains are found in a broad range of cell surface and secreted proteins, where they play key physiological roles. In addition, alterations in mucin expression and glycosylation are common in a variety of human diseases, such as cancer, cystic fibrosis, and inflammatory bowel diseases. These correlations have been challenging to uncover and establish because tools that specifically probe mucin domains are lacking. Here, we present a panel of bacterial proteases that cleave mucin domains via distinct peptide- and glycan-based motifs, generating a diverse enzymatic toolkit for mucin-selective proteolysis. By mutating catalytic residues of two such enzymes, we engineered mucin-selective binding agents with retained glycoform preferences. StcEE447D is a pan-mucin stain derived from enterohemorrhagic Escherichia coli that is tolerant to a wide range of glycoforms. BT4244E575A derived from Bacteroides thetaiotaomicron is selective for truncated, asialylated Core 1 structures commonly associated with malignant and pre-malignant tissues. We demonstrated that these catalytically inactive point mutants enable robust detection and visualization of mucin-domain glycoproteins by flow cytometry, Western blot, and immunohistochemistry. Application of our enzymatic toolkit to ovarian cancer patient ascites fluid and tissue slices facilitated characterization of patients based on differences in mucin cleavage and expression patterns.

Keywords

O-glycosylation
mucin
mucinase
protease
mass spectrometry
immunohistochemistry

Supplementary materials

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Dataset S1 BT4244 ConsensusSeq
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Dataset S2 AM0627 ConsensusSeq
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Dataset S3 Pic ConsensusSeq
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Dataset S4 ZmpC ConsensusSeq
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Dataset S5 AM0908 ConsensusSeq
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Dataset S6 AM1514 ConsensusSeq
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Dataset S7 TagA ConsensusSeq
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