Engineering Orthogonal Polypeptide GalNAc-Transferase and UDP-Sugar Pairs

Choi, Jun Won; Wagner, Lauren J. S.; Timmermans, Suzanne B. P. E.; Malaker, Stacy A.; Schumann, Benjamin; Gray, Melissa A.; Debets, Marjoke F.; Takashima, Megumi; Gehring, Jase; Bertozzi, Carolyn R.

doi:10.1021/jacs.9b04695

Cited by 63 publications

(71 citation statements)

References 73 publications

(179 reference statements)

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“…Further complexity is added by the interplay of 20 GalNAc transferase (GalNAc-T1…T20) isoenzymes that mediate the first O-GalNAc biosynthesis step (22, 23). In a “bump-and-hole” (BH) approach, we have recently engineered GalNAc-Ts to carry a double mutation to preferentially accept UDP-GalNAc analogs with bulky chemical, editable tags (24, 25). Although this technique produced bioorthogonal reporters with great specificity for particular GalNAc-T isoenzymes, epimerization of GalNAc analogs by GALE was still a challenge and resulted in background N-glycan labeling (25).…”

Section: Introductionmentioning

confidence: 99%

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: Introductionmentioning

confidence: 99%

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

Debets¹,

Tastan

Wisnovsky³

et al. 2020

Preprint

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“…Subsequent epimerizations (to generate the galactose and mannose derivatives 4 and 5 , respectively) and further elaboration to sialic acids ( 6 ) and glycoconjugates can also be achieved enzymatically. However, there remains a gap in the enzyme toolkit in that the acylation of glucosamine ( 2 ) needs to be performed chemically, requiring the activation of carboxylic acids or stoichiometric coupling agents and protecting strategies …”

Section: Methodsmentioning

confidence: 99%

An Enzymatic N‐Acylation Step Enables the Biocatalytic Synthesis of Unnatural Sialosides

et al. 2020

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Chitin is one of the most abundant and cheaply available biopolymers in Nature. Chitin has become a valuable starting material for many biotechnological products through manipulation of its N‐acetyl functionality, which can be cleaved under mild conditions using the enzyme family of de‐N‐acetylases. However, the chemoselective enzymatic re‐acylation of glucosamine derivatives, which can introduce new stable functionalities into chitin derivatives, is much less explored. Herein we describe an acylase (CmCDA from Cyclobacterium marinum) that catalyzes the N‐acylation of glycosamine with a range of carboxylic acids under physiological reaction conditions. This biocatalyst closes an important gap in allowing the conversion of chitin into complex glycosides, such as C5‐modified sialosides, through the use of highly selective enzyme cascades.

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“…We next sought to confirm that DM-GalNAcTs localize to the Golgi compartment and glycosylate alkyne chain led to substantial labeling, consistent with 4 being a substrate for WT-GalNAcTs (8,26). These results were confirmed using soluble GalNAcTs and a membrane fraction of nontransfected cells (Fig.…”

Section: Dm-galnacts Glycosylate Membrane Proteinsmentioning

confidence: 98%

“…1B) re-programmed GalNAcTs to accept alkynecontaining uridine diphosphate (UDP)-GalNAc analogs such as compounds 1-4 instead of the native substrate UDP-GalNAc ( Fig. 1B) (8). We endowed living cells with the capacity to biosynthesize a UDP-GalNAc analog that was complementary to engineered DM-GalNAcTs.…”

mentioning

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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Engineering Orthogonal Polypeptide GalNAc-Transferase and UDP-Sugar Pairs

Cited by 63 publications

References 73 publications

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

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

An Enzymatic N‐Acylation Step Enables the Biocatalytic Synthesis of Unnatural Sialosides

Chemical precision glyco-mutagenesis by glycosyltransferase engineering in living cells

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