Toward the assembly and characterization of an encoded library hit confirmation platform: Bead-Assisted Ligand Isolation Mass Spectrometry (BALI-MS)

化学 DNA 计算生物学 质谱法 DNA测序 脱氧核酶 条形码 序列(生物学) 组合化学 色谱法 生物化学 计算机科学 生物 操作系统
作者
Anokha S. Ratnayake,Mark E. Flanagan,Timothy L. Foley,Scott L. Hultgren,Justin Bellenger,Justin I. Montgomery,Manjinder S. Lall,Бо Лю,Tim F. Ryder,Dominik K. Kölmel,Andre Shavnya,Xidong Feng,Bruce A. Lefker,Laura J. Byrnes,Parag V. Sahasrabudhe,Kathleen A. Farley,Shi Chen,Jinqiao Wan
出处
期刊:Bioorganic & Medicinal Chemistry [Elsevier BV]
卷期号:41: 116205-116205 被引量:18
标识
DOI:10.1016/j.bmc.2021.116205
摘要

Abstract The ability to predict chemical structure from DNA sequence has to date been a necessary cornerstone of DNA-encoded library technology. DNA-encoded libraries (DELs) are typically screened by immobilized affinity selection and enriched library members are identified by counting the number of times an individual compound’s sequence is observed in the resultant dataset. Those with high signal reads (DEL hits) are subsequently followed up through off-DNA synthesis of the predicted small molecule structures. However, hits followed-up in this manner often fail to translate to confirmed ligands. To address this low conversion rate of DEL hits to off-DNA ligands, we have developed an approach that eliminates the reliance on chemical structure prediction from DNA sequence. Here we describe our method of combining non-combinatorial resynthesis on-DNA following library procedures as a rapid means to assess the probable molecules attached to the DNA barcode. Furthermore, we apply our Bead-Assisted Ligand Isolation Mass Spectrometry (BALI-MS) technique to identify the true binders found within the mixtures of on-DNA synthesis products. Finally, we describe a Normalized Enrichment (NE) metric that allows for the quantitative assessment of affinity selection in these studies. We exemplify how this combined approach enables the identification of putative hit matter against a clinically relevant therapeutic target bisphosphoglycerate mutase, BPGM.
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