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生物层干涉技术为检测微生物提取物中的 DNA 结合小分子提供了一种可靠的方法。

Biolayer interferometry provides a robust method for detecting DNA binding small molecules in microbial extracts.

机构信息

Department of Chemistry, Oregon State University, Corvallis, OR, 97331, USA.

Whitney Laboratory for Marine Bioscience, Department of Chemistry, University of Florida, St. Augustine, FL, 32080, USA.

出版信息

Anal Bioanal Chem. 2021 Feb;413(4):1159-1171. doi: 10.1007/s00216-020-03079-5. Epub 2020 Nov 25.

DOI:10.1007/s00216-020-03079-5
PMID:33236226
Abstract

DNA replication is an exceptional point of therapeutic intervention for many cancer types and several small molecules targeting DNA have been developed into clinically used antitumor agents. Many of these molecules are naturally occurring metabolites from plants and microorganisms, such as the widely used chemotherapeutic doxorubicin. While natural product sources contain a vast number of DNA binding small molecules, isolating and identifying these molecules is challenging. Typical screening campaigns utilize time-consuming bioactivity-guided fractionation approaches, which use sequential rounds of cell-based assays to guide the isolation of active compounds. In this study, we explore the use of biolayer interferometry (BLI) as a tool for rapidly screening natural product sources for DNA targeting small molecules. We first verified that BLI robustly detected DNA binding using designed GC- and AT-rich DNA oligonucleotides with known DNA intercalating, groove binding, and covalent binding agents including actinomycin D (1), doxorubicin (2), ethidium bromide (3), propidium iodide (4), Hoechst 33342 (5), and netropsin (6). Although binding varied with the properties of the oligonucleotides, measured binding affinities agreed with previously reported values. We next utilized BLI to screen over 100 bacterial extracts from our microbial library for DNA binding activity and found three highly active extracts. Binding-guided isolation was used to isolate the active principle component from each extract, which were identified as echinomycin (8), actinomycin V (9), and chartreusin (10). This biosensor-based DNA binding screen is a novel, low-cost, easy to use, and sensitive approach for medium-throughput screening of complex chemical libraries. Graphical abstract.

摘要

DNA 复制是许多癌症类型治疗干预的一个特殊点,已经开发出几种针对 DNA 的小分子药物作为临床抗肿瘤药物。这些分子中的许多是来自植物和微生物的天然存在的代谢物,例如广泛使用的化疗药物多柔比星。虽然天然产物来源含有大量与 DNA 结合的小分子,但分离和鉴定这些分子具有挑战性。典型的筛选活动利用耗时的基于生物活性的分级分离方法,该方法使用基于细胞的测定的连续轮次来指导活性化合物的分离。在这项研究中,我们探索了使用生物层干涉(BLI)作为快速筛选天然产物来源中 DNA 靶向小分子的工具。我们首先通过使用设计的富含 GC 和富含 AT 的 DNA 寡核苷酸验证了 BLI 可以可靠地检测 DNA 结合,这些寡核苷酸具有已知的 DNA 嵌入、沟结合和共价结合剂,包括放线菌素 D(1)、多柔比星(2)、溴化乙锭(3)、碘化丙啶(4)、Hoechst 33342(5)和 netropsin(6)。尽管结合随寡核苷酸的性质而变化,但测量的结合亲和力与先前报道的值一致。接下来,我们利用 BLI 从我们的微生物文库中筛选了 100 多个细菌提取物的 DNA 结合活性,发现了三个高度活跃的提取物。结合导向分离用于从每个提取物中分离出活性成分,这些成分被鉴定为表柔比星(8)、放线菌素 V(9)和沙雷菌素(10)。这种基于生物传感器的 DNA 结合筛选是一种新颖、低成本、易于使用且灵敏的方法,适用于复杂化学文库的高通量筛选。

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