Electrophilic probes for deciphering substrate recognition by O-GlcNAc transferase

Hu, Chia‐Wei; Worth, Matthew; Fan, Dacheng; Li, Baobin; Li, Hao; Lü, Lei; Zhong, Xiaofang; Lin, Ziqing; Wei, Liming; Ge, Ying; Jiang, Jiaoyang

doi:10.1038/nchembio.2494

Cited by 30 publications

(33 citation statements)

References 57 publications

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“…An OGT mutant construct consisting of alanine in place of these 5 asparagine residues (5N5A) retained activity toward short peptides but impaired modification of proteins [10], supporting the importance of these residues in indiscriminate recognition of the polypeptide backbone of proteins distant from the site of glycosylation. In a different approach, the Jiang group developed a GlcNAc electrophilic probe (GEP) that consists of a UDP-GlcNAc analog containing an allyl chloride electrophile extending as an N-acyl group from the 2-amino position [12]. This GEP was used to discern whether mutations in OGT affected sugar binding or protein acceptor binding and glycosylation by examining its relative partitioning to OGT (C917) or the acceptor protein.…”

Section: Ogt Structure and Polypeptide Acceptor Specificitymentioning

confidence: 99%

Molecular mechanisms regulating O-linked N-acetylglucosamine (O-GlcNAc)–processing enzymes

King

Males

Davies

et al. 2019

Current Opinion in Chemical Biology

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The post-translational modification of proteins by O-linked N-acetylglucosamine (O-GlcNAc) dynamically programs cellular physiology to maintain homeostasis and tailor biochemical pathways to meet context-dependant cellular needs. Despite diverse roles for O-GlcNAc, only two enzymes act antagonistically to govern its cycling; O-GlcNAc transferase (OGT) installs the monosaccharide on target proteins and O-GlcNAc hydrolase (OGA) removes it. Recent literature has exposed a network of mechanisms regulating these two enzymes to choreograph global, and target-specific, O-GlcNAc cycling in response to cellular stress and nutrient availability. Herein, we amalgamate these emerging mechanisms from a structural and molecular perspective to explore how the cell exerts fine control to regulate O-GlcNAcylation of diverse proteins in a selective fashion. Papers of particular interest, published within the period of review, have been highlighted as: *of special interest ** of outstanding interest **[3] An important paper in the field. The authors provide unambiguous evidence for mutations in ogt implicated in XLID influencing OGT function. Despite largely normal global O-GlcNAc levels, significant changes in gene transcription are observed. Furthermore, a compensatory mechanism to maintain global O-GlcNAc levels involving OGT-mSin3A-HDAC1 dependant transcriptional repression at the OGA promoter is proposed. *[6] The authors develop a systematic platform for glycosylation sequence characterization and optimization and use this method to characterize OGT sequence preference. This analysis revealed a surprising preference for an aromatic residue at the-4 subsite. *[10] An asparagine ladder in the TPR domains mediates OGT interaction with protein substrates. * [12] New chemical biology tools to identify features of OGT responsible for substrate targeting. This method uncovered a patch of residues lining the inner surface of the N-terminal domain that contribute to interaction with multiple substrates. **[13] A nice structural study defines the effect of XLID-associated OGT mutation L254F as distorting the TPR helix. * [27] mOGT was shown to be catalytically active in vivo and plays an important role in supporting mitochondrial structure and function. **[28] A fundamental advance in discovery of the OGT NLS and the effects of S389 O-GlcNAcylation and interaction with importin α5 for nuclear import. *[35] The authors demonstrate that OGT is enriched in the post-synaptic density of excitatory neuronal synapses whereby it regulates synapse maturation. *[37] Upon glucagon-induced calcium signalling CamKII phosphorylates OGT at S20, which induces O-GlcNAc modification of Ulk proteins through potentiation of AMPKdependant phosphorylation. **[38] Chk1 phosphorylates OGT S20, and this modification regulates OGT localization to the mid-body and regulation of vimentin bridge formation and severing during mitosis. *[39] LSD2 was shown to act as an E3 ligase to ubiquitinylate OGT and thereby facilitate its UPS mediated degradation. **[43] Circad...

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Section: Ogt Structure and Polypeptide Acceptor Specificitymentioning

confidence: 99%

Molecular mechanisms regulating O-linked N-acetylglucosamine (O-GlcNAc)–processing enzymes

King

Males

Davies

et al. 2019

Current Opinion in Chemical Biology

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“…In combination with structureguidedm utagenesis, this new probe can rapidly assesst he role of specific OGT residues in bindings ugar donor compared to acceptorsubstrates (Figure 3). [69] GEP1 contains an allyl chloride electrophile that extends from the N-acetyl group of UDP-GlcNAc. In the presence of protein substrates, this probe can be used as ar egular sugar donor to conduct glycosylation by OGT.I nt he absence of acceptor substrates, this probe can efficiently label OGT active-site residue C917 to generateacovalent modification on OGT.T he binding ability of OGT toward sugar and protein substrates can be evaluated by varying the level of probe modified protein and OGT.T his can be reported by using click-chemistry conjugation of an alkyne fluorophore with the 6'-azido group on am odified GEP1 probe "GEP1A"i n af luorescence assay (Figure 3).…”

Section: Microarrays To Elucidate the Substrate Preferences Of Ogt Anmentioning

confidence: 99%

“…Following brief preincubation with OGT,G EP1 wasa ble to in situ crosslink OGT with over 100 proteins in cell lysates (Figure 3). [69] Most of thesec rosslinked proteins were reported to be O-GlcNAcylated, and dozens of possible new OGT substrate proteins were also identified. The crosslinking assay of GEP1 can facilitate the identification of novel OGT substrates and could be optimized for characterizing the binding mode of particular substrates with OGT.I ts hould be noted that this probe is not currently applicable in cells, and the electrophiles and assay conditions might requireo ptimization for different substrates.…”

Section: Microarrays To Elucidate the Substrate Preferences Of Ogt Anmentioning

confidence: 99%

“…A UDP‐GlcNAc analogue called GlcNAc electrophilic probe 1 (GEP1) that addresses this limitation was recently reported. In combination with structure‐guided mutagenesis, this new probe can rapidly assess the role of specific OGT residues in binding sugar donor compared to acceptor substrates (Figure ) . GEP1 contains an allyl chloride electrophile that extends from the N ‐acetyl group of UDP‐GlcNAc.…”

Section: Introductionmentioning

confidence: 99%

“…GEP1 can also potentially stabilize OGT–protein substrate complexes to facilitate investigation of their interactions. Following brief preincubation with OGT, GEP1 was able to in situ crosslink OGT with over 100 proteins in cell lysates (Figure ) . Most of these crosslinked proteins were reported to be O‐GlcNAcylated, and dozens of possible new OGT substrate proteins were also identified.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Chemical and Biochemical Strategies To Explore the Substrate Recognition of O‐GlcNAc‐Cycling Enzymes

Worth

et al. 2018

ChemBioChem

Self Cite

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The O-linked N-acetylglucosamine (O-GlcNAc) modification is an essential component in cell regulation. A single pair of human enzymes conducts this modification dynamically on a broad variety of proteins: O-GlcNAc transferase (OGT) adds the GlcNAc residue and O-GlcNAcase (OGA) hydrolyzes it. This modification is dysregulated in many diseases, but its exact effect on particular substrates remains unclear. In addition, no apparent sequence motif has been found in the modified proteins, and the factors controlling the substrate specificity of OGT and OGA are largely unknown. In this minireview, we will discuss recent developments in chemical and biochemical methods toward addressing the challenge of OGT and OGA substrate recognition. We hope that the new concepts and knowledge from these studies will promote research in this area to advance understanding of O-GlcNAc regulation in health and disease.

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C‐Terminal Tag Location Hampers in Vitro Profiling of OGT Peptide Substrates by mRNA Display

et al. 2020

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O‐GlcNAc transferase (OGT) is the only enzyme that catalyzes the post‐translational modification of proteins at Ser/Thr with a single β‐N‐acetylglucosamine (O‐GlcNAcylation). Its activity has been associated with chronic diseases such as cancer, diabetes and neurodegenerative disease. Although numerous OGT substrates have been identified, its accepted substrate scope can still be refined. We report here an attempt to better define the peptide‐recognition requirements of the OGT active site by using mRNA display, taking advantage of its extremely high throughput to assess the substrate potential of a library of all possible nonamer peptides. An antibody‐based selection process is described here that is able to enrich an OGT substrate peptide from such a library, but with poor absolute recovery. Following four rounds of selection for O‐GlcNAcylated peptides, sequencing revealed 14 peptides containing Ser/Thr, but these were shown by luminescence‐coupled assays and peptide microarray not to be OGT substrates. By contrast, subsequent testing of an N‐terminal tag approach showed exemplary recovery. Our approach demonstrates the power of genetically encoded libraries for selection of peptide substrates, even from a very low initial starting abundance and under suboptimal conditions, and emphasizes the need to consider the binding biases of antibodies and both C‐ and N‐terminal tags in profiling peptide substrates by high‐throughput display.

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Electrophilic probes for deciphering substrate recognition by O-GlcNAc transferase

Cited by 30 publications

References 57 publications

Molecular mechanisms regulating O-linked N-acetylglucosamine (O-GlcNAc)–processing enzymes

Molecular mechanisms regulating O-linked N-acetylglucosamine (O-GlcNAc)–processing enzymes

Chemical and Biochemical Strategies To Explore the Substrate Recognition of O‐GlcNAc‐Cycling Enzymes

C‐Terminal Tag Location Hampers in Vitro Profiling of OGT Peptide Substrates by mRNA Display

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