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Reactivity-dependent profiling of RNA 5-methylcytidine dioxygenases

A. Emilia Arguello, Ang Li, Xuemeng Sun, Tanner W. Eggert, Elisabeth Mairhofer and Ralph E. Kleiner ()
Additional contact information
A. Emilia Arguello: Princeton University
Ang Li: Princeton University
Xuemeng Sun: Princeton University
Tanner W. Eggert: Princeton University
Elisabeth Mairhofer: Princeton University
Ralph E. Kleiner: Princeton University

Nature Communications, 2022, vol. 13, issue 1, 1-17

Abstract: Abstract Epitranscriptomic RNA modifications can regulate fundamental biological processes, but we lack approaches to map modification sites and probe writer enzymes. Here we present a chemoproteomic strategy to characterize RNA 5-methylcytidine (m5C) dioxygenase enzymes in their native context based upon metabolic labeling and activity-based crosslinking with 5-ethynylcytidine (5-EC). We profile m5C dioxygenases in human cells including ALKBH1 and TET2 and show that ALKBH1 is the major hm5C- and f5C-forming enzyme in RNA. Further, we map ALKBH1 modification sites transcriptome-wide using 5-EC-iCLIP and ARP-based sequencing to identify ALKBH1-dependent m5C oxidation in a variety of tRNAs and mRNAs and analyze ALKBH1 substrate specificity in vitro. We also apply targeted pyridine borane-mediated sequencing to measure f5C sites on select tRNA. Finally, we show that f5C at the wobble position of tRNA-Leu-CAA plays a role in decoding Leu codons under stress. Our work provides powerful chemical approaches for studying RNA m5C dioxygenases and mapping oxidative m5C modifications and reveals the existence of novel epitranscriptomic pathways for regulating RNA function.

Date: 2022
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DOI: 10.1038/s41467-022-31876-2

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