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Chemoenzymatic Site-Specific Labeling of DNA and RNA Oligonucleotides by Leveraging the Exclusive Reactivity of Glycine-Modified Nucleotide Analogs

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dc.contributor.author PAL, ARINDAM en_US
dc.contributor.author PHADTE, APEKSHA A. en_US
dc.contributor.author KHAMARI, ROSHNI R. en_US
dc.contributor.author Rai,Vishal en_US
dc.contributor.author SRIVATSAN, SEERGAZHI G. en_US
dc.date.accessioned 2026-01-30T06:35:08Z
dc.date.available 2026-01-30T06:35:08Z
dc.date.issued 2026-01 en_US
dc.identifier.citation Bioconjugate Chemistry, 37(01), 52–62. en_US
dc.identifier.issn 1043-1802 en_US
dc.identifier.issn 1520-4812 en_US
dc.identifier.uri https://doi.org/10.1021/acs.bioconjchem.5c00473 en_US
dc.identifier.uri http://dr.iiserpune.ac.in:8080/xmlui/handle/123456789/10675
dc.description.abstract The landscape of nucleic acid modification technologies is rapidly evolving, with chemoselective postsynthetic labeling strategies emerging as indispensable chemical tools for generating functionalized oligonucleotides (ONs). These methods greatly rely on reactions between groups such as amine/thiol or clickable handles like azide/alkyne with cognate reaction partners. However, achieving precise covalent labeling in the presence of competing functionalities and preserving ON integrity, particularly in RNA, presents significant challenges. Here, we present an innovative chemoenzymatic platform for DNA and RNA labeling that leverages the unique chemoselective reactivity of terminal glycine-modified (Gly-tag) nucleotide analogs with o-substituted benzaldehyde substrates equipped with strategic hydrogen bond acceptors. The Gly-tagged nucleotide analogs (dGTTP and GUTP) serve as excellent substrates for DNA and RNA polymerases and terminal uridylyl transferase, thereby allowing the incorporation of the reactive Gly-tag at desired positions into DNA and RNA ONs. Notably, o-substituted benzaldehyde substrates, bearing a proximal oxyacetamide moiety, facilitate efficient postenzymatic conjugation, enabling site-selective installation of functionalities including affinity tags, fluorescent probes and clickable groups with good yields and remarkable selectivity. Taken together, this chemoenzymatic methodology represents a new toolkit for late-stage ON labeling, opening up new avenues for advancing nucleic acid applications in diagnostics and biotechnology. en_US
dc.language.iso en en_US
dc.publisher American Chemical Society en_US
dc.subject Genetics en_US
dc.subject Labeling en_US
dc.subject Monomers en_US
dc.subject Nucleic acids en_US
dc.subject Peptides and proteins en_US
dc.subject 2026-JAN-WEEK4 en_US
dc.subject TOC-JAN-2026 en_US
dc.subject 2026 en_US
dc.title Chemoenzymatic Site-Specific Labeling of DNA and RNA Oligonucleotides by Leveraging the Exclusive Reactivity of Glycine-Modified Nucleotide Analogs en_US
dc.type Article en_US
dc.contributor.department Dept. of Chemistry en_US
dc.identifier.sourcetitle Bioconjugate Chemistry en_US
dc.publication.originofpublisher Foreign en_US


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