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DNA 四重螺旋-双链结构增强对一种草药化合物姜黄素的识别。

Enhanced Recognition of a Herbal Compound Epiberberine by a DNA Quadruplex-Duplex Structure.

机构信息

School of Medicine, The Chinese University of Hong Kong, Shenzhen (CUHK-Shenzhen), Shenzhen 518172, Guangdong, P. R. China.

Division of Chemistry and Biological Chemistry, School of Physical and Mathematical Sciences, Nanyang Technological University, 637371 Singapore.

出版信息

Anal Chem. 2024 Aug 13;96(32):13174-13184. doi: 10.1021/acs.analchem.4c02054. Epub 2024 Aug 2.

DOI:10.1021/acs.analchem.4c02054
PMID:39093925
Abstract

The small molecule epiberberine (EPI) is a natural alkaloid with versatile bioactivities against several diseases including cancer and bacterial infection. EPI can induce the formation of a unique binding pocket at the 5' side of a human telomeric G-quadruplex (HTG) sequence with four telomeric repeats (Q4), resulting in a nanomolar binding affinity ( approximately 26 nM) with significant fluorescence enhancement upon binding. It is important to understand (1) how EPI binding affects HTG structural stability and (2) how enhanced EPI binding may be achieved through the engineering of the DNA binding pocket. In this work, the EPI-binding-induced HTG structure stabilization effect was probed by a peptide nucleic acid (PNA) invasion assay in combination with a series of biophysical techniques. We show that the PNA invasion-based method may be useful for the characterization of compounds binding to DNA (and RNA) structures under physiological conditions without the need to vary the solution temperature or buffer components, which are typically needed for structural stability characterization. Importantly, the combination of theoretical modeling and experimental quantification allows us to successfully engineer Q4 derivative Q4-ds-A by a simple extension of a duplex structure to Q4 at the 5' end. Q4-ds-A is an excellent EPI binder with a of 8 nM, with the binding enhancement achieved through the preformation of a binding pocket and a reduced dissociation rate. The tight binding of Q4 and Q4-ds-A with EPI allows us to develop a novel magnetic bead-based affinity purification system to effectively extract EPI from (Huang Lian) extracts.

摘要

小分子小檗碱(EPI)是一种天然生物碱,具有多种生物活性,可对抗多种疾病,包括癌症和细菌感染。EPI 可以在人类端粒 G-四链体(HTG)序列的 5'侧形成一个独特的结合口袋,该序列具有四个端粒重复(Q4),导致与结合时具有显著荧光增强的纳摩尔结合亲和力(约 26 nM)。了解(1)EPI 结合如何影响 HTG 结构稳定性,以及(2)如何通过工程化 DNA 结合口袋来实现增强的 EPI 结合非常重要。在这项工作中,通过肽核酸(PNA)入侵测定法结合一系列生物物理技术来探测 EPI 结合诱导的 HTG 结构稳定化效应。我们表明,基于 PNA 入侵的方法可能可用于在生理条件下表征与 DNA(和 RNA)结构结合的化合物,而无需改变溶液温度或缓冲成分,这些通常是结构稳定性表征所必需的。重要的是,理论建模和实验量化的结合使我们能够通过简单地将双链结构扩展到 5'端的 Q4 来成功地对 Q4 衍生物 Q4-ds-A 进行工程设计。Q4-ds-A 是一种极好的 EPI 结合物,具有 8 nM 的 Ki 值,通过预形成结合口袋和降低解离速率来实现结合增强。Q4 和 Q4-ds-A 与 EPI 的紧密结合使我们能够开发一种新型的基于磁珠的亲和纯化系统,以有效地从黄连提取物中提取 EPI。

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