The mucin-selective protease StcE enables molecular and functional analysis of human cancer-associated mucins

Malaker, Stacy A.; Pedram, Kayvon; Ferracane, Michael J.; Bensing, Barbara A.; Krishnan, Venkatesh; Pett, Christian; Yu, Jin; Woods, Elliot C.; Kramer, Jessica R.; Westerlind, Ulrika; Dorigo, Oliver; Bertozzi, Carolyn R.

doi:10.1073/pnas.1813020116

Cited by 211 publications

(328 citation statements)

References 81 publications

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“…To assess labeling specificity, we also tested glycoprotein susceptibility towards hydrolytic enzymes. We treated samples with the mucinase StcE that specifically digests highly O-GalNAcylated mucin domains, or with sialidase that removes sialic acid from glycoconjugates (36). Following StcE treatment, the most intense bands labeled by both caged GalNAzMe-1-phosphate 11 and Ac 4 GalNAz feeding had disappeared.…”

Section: Resultsmentioning

confidence: 99%

“…Supernatant was transferred to a new plate and BCA was used to measure protein concentration. For enzyme treatment, equal amounts of protein (typically 15 µg) were diluted to 40 µL with Lysis Buffer or PBS, treated with either SialEXO (4 µL of a 4 U/µL solution in 50 mM Tris-HCl (pH 6.5), Genovis, Lund, Sweden) or the glycoprotease StcE (50 nM in PBS) (19) and incubated for 2 h at 37 °C. The reaction was quenched by heating to 95 °C for 10 s with subsequent cooling at 4 °C.…”

Section: Supporting Informationmentioning

confidence: 99%

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Metabolic precision labeling enables selective probing of O-linkedN-acetylgalactosamine glycosylation

Debets¹,

Tastan

Wisnovsky³

et al. 2020

Preprint

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38Protein glycosylation events that happen early in the secretory pathway are often dysregulated during 39 tumorigenesis. These events can be probed, in principle, by monosaccharides with bioorthogonal tags that 40 would ideally be specific for distinct glycan subtypes. However, metabolic interconversion into other 41 monosaccharides drastically reduces such specificity in the living cell. Here, we use a structure-based 42 design process to develop the monosaccharide probe GalNAzMe that is specific for cancer-relevant 43

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Section: Resultsmentioning

confidence: 99%

Section: Supporting Informationmentioning

confidence: 99%

Metabolic precision labeling enables selective probing of O-linkedN-acetylgalactosamine glycosylation

Debets¹,

Tastan

Wisnovsky³

et al. 2020

Preprint

Self Cite

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show abstract

“…Empowered by the proximity labeling approach, we now have generated a priority list of proteins that will be the subject of future work to further reveal the "professional glycoprotein ligands" [14] required for the functional activation of HSCs. Already, preliminary work has shown that basigin plays an active role in hepatic fibrosis [45], and our own work will delve deeper into the molecular nature of the galectin-3-basigin interaction.…”

Section: Discussionmentioning

confidence: 99%

Mapping glycan-mediated galectin-3 interactions by live cell proximity labeling

Joeh

O’Leary

et al. 2020

Preprint

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Galectin-3 is a glycan-binding protein (GBP) that binds b-galactoside glycan structures to orchestrate a variety of important biological events, including the activation of hepatic stellate cells to cause hepatic fibrosis. While the requisite glycan epitopes needed to bind galectin-3 have long been elucidated, the cellular glycoproteins that bear these glycan signatures remain unknown. Given the importance of the threedimensional arrangement of glycans in dictating GBP interactions, strategies that allow the identification of GBP receptors in live cells, where the native glycan presentation and glycoprotein expression are preserved, possess significant advantages over static and artificial systems. Here, we describe the integration of a proximity labeling method and quantitative mass spectrometry to map the glycan and glycoprotein interactors for galectin-3 in live hepatic stellate cells. Understanding the identity of the glycoproteins and defining the structures of the glycans required for galectin-3 mediated hepatic stellate cell activation will empower efforts to design and develop selective therapeutics to mitigate hepatic fibrosis. SignificanceBecause of the weak interactions between individual glycan-binding proteins (GBP), such as galectin-3, and glycans, strategies that allow the direct interrogation of these interactions in living cells remain limited.Thus, the glycan and glycoprotein ligands that are physiologically relevant for galectin-3 binding are insufficiently described. Here, we used a proximity labeling approach that catalytically tags interactors for galectin-3 and identified its pertinent glycan and glycoprotein counter-receptors in live hepatic stellate cells.This study demonstrates that proximity labeling is a powerful tool for mapping GBP complexes in living cells, and when coupled with chemical inhibitors, it can discriminate between protein-protein and proteinglycan interactions. Graphical Abstract

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“…The era of quantitative biology demands great specificity in tools to probe cellular processes or expressed antigens. Biological tools, including antibodies, lectins, engineered binding proteins, or 10 silenced hydrolases have been employed to profile or isolate cellular glycans (45,50). While powerful probes, these proteins suffer from various drawbacks, including the dependence of binding on the structural context or the requirement to simplify glycans before performing binding studies.…”

Section: Discussionmentioning

confidence: 99%

Chemical precision glyco-mutagenesis by glycosyltransferase engineering in living cells

Schumann

Malaker

Wisnovsky

et al. 2019

Preprint

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AbstractStudying posttranslational modifications classically relies on experimental strategies that oversimplify the complex biosynthetic machineries of living cells. Protein glycosylation contributes to essential biological processes, but correlating glycan structure, underlying protein and disease-relevant biosynthetic regulation is currently elusive. Here, we engineer living cells to tag glycans with editable chemical functionalities while providing information on biosynthesis, physiological context and glycan fine structure. We introduce a non-natural substrate biosynthetic pathway and use engineered glycosyltransferases to incorporate chemically tagged sugars into the cell surface glycome of the living cell. We apply the strategy to a particularly redundant yet disease-relevant human glycosyltransferase family, the polypeptide N-acetylgalactosaminyl transferases. This approach bestows a gain-of-function modification on cells where the products of individual glycosyltransferases can be selectively characterized or manipulated at will.

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The mucin-selective protease StcE enables molecular and functional analysis of human cancer-associated mucins

Cited by 211 publications

References 81 publications

Metabolic precision labeling enables selective probing of O-linkedN-acetylgalactosamine glycosylation

Metabolic precision labeling enables selective probing of O-linkedN-acetylgalactosamine glycosylation

Mapping glycan-mediated galectin-3 interactions by live cell proximity labeling

Chemical precision glyco-mutagenesis by glycosyltransferase engineering in living cells

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