| Literature DB >> 34267887 |
Bing Xia1, G Joseph Franklin1, Xiaojie Lu1, Katie L Bedard1, LaShadric C Grady1, Jennifer D Summerfield1, Eric X Shi1, Bryan W King2, Kenneth E Lind1, Cynthia Chiu1, Eleanor Watts1, Vera Bodmer1, Xiaopeng Bai1, Lisa A Marcaurelle1.
Abstract
DNA-encoded library (DEL) technology is a powerful platform for hit identification in academia and the pharmaceutical industry. When conducting off-DNA resynthesis hit confirmation after affinity selection, PCR/sequencing, and data analysis, one typically assumes a "one-to-one" relationship between the DNA tag and the chemical structure of the attached small-molecule it encodes. Because library synthesis often yields a mixture, this approximation increases the risk of overlooking positive discoveries and valuable information. To address this issue, we apply a library synthesis "recipe" strategy for on-DNA resynthesis using a cleavable linker, followed by direct affinity selection mass spectrometry (AS-MS) evaluation and identification of binder(s) from the released small-molecule mixture. We validate and showcase this approach employing the receptor-interacting-protein kinase 2 (RIP2) DEL campaign. We also designed and developed two cleavable linkers to enable this method, a photocleavable linker (nitrophenyl-based) and acid-labile linker (tetrahydropyranyl ether). The strategy provides an effective means of hit identification and rapid determination of key active component(s) of the mixture.Entities:
Year: 2021 PMID: 34267887 PMCID: PMC8274064 DOI: 10.1021/acsmedchemlett.1c00156
Source DB: PubMed Journal: ACS Med Chem Lett ISSN: 1948-5875 Impact factor: 4.632