Transcriptome-Wide Mapping of Small-Molecule RNA-Binding Sites in Cells Informs an Isoform-Specific Degrader of QSOX1 mRNA

化学 核糖核酸 转录组 基因亚型 信使核糖核酸 生物化学 基因表达 基因
作者
Yuquan Tong,Quentin M. R. Gibaut,Warren B. Rouse,Jessica L. Childs‐Disney,Blessy M. Suresh,Daniel Abegg,Shruti Choudhary,Yoshihiro Akahori,Alexander Adibekian,Walter N. Moss,Matthew D. Disney
出处
期刊:Journal of the American Chemical Society [American Chemical Society]
卷期号:144 (26): 11620-11625 被引量:60
标识
DOI:10.1021/jacs.2c01929
摘要

The interactions between cellular RNAs in MDA-MB-231 triple negative breast cancer cells and a panel of small molecules appended with a diazirine cross-linking moiety and an alkyne tag were probed transcriptome-wide in live cells. The alkyne tag allows for facile pull-down of cellular RNAs bound by each small molecule, and the enrichment of each RNA target defines the compound's molecular footprint. Among the 34 chemically diverse small molecules studied, six bound and enriched cellular RNAs. The most highly enriched interaction occurs between the novel RNA-binding compound F1 and a structured region in the 5' untranslated region of quiescin sulfhydryl oxidase 1 isoform a (QSOX1-a), not present in isoform b. Additional studies show that F1 specifically bound RNA over DNA and protein; that is, we studied the entire DNA, RNA, and protein interactome. This interaction was used to design a ribonuclease targeting chimera (RIBOTAC) to locally recruit Ribonuclease L to degrade QSOX1 mRNA in an isoform-specific manner, as QSOX1-a, but not QSOX1-b, mRNA and protein levels were reduced. The RIBOTAC alleviated QSOX1-mediated phenotypes in cancer cells. This approach can be broadly applied to discover ligands that bind RNA in cells, which could be bioactive themselves or augmented with functionality such as targeted degradation.
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