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通过选择性碳纳米管组装实现小分子连接DNA的末端保护,用于蛋白质结合的灵敏电化学检测。

Terminal protection of small-molecule-linked DNA for sensitive electrochemical detection of protein binding via selective carbon nanotube assembly.

作者信息

Wu Zhan, Zhen Zhen, Jiang Jian-Hui, Shen Guo-Li, Yu Ru-Qin

机构信息

State Key Laboratory of Chemo/Bio-Sensing and Chemometrics, College of Chemistry and Chemical Engineering, Hunan University, Changsha, 410082, PR China.

出版信息

J Am Chem Soc. 2009 Sep 2;131(34):12325-32. doi: 10.1021/ja9038054.

DOI:10.1021/ja9038054
PMID:19655753
Abstract

Small-molecule-linked DNA has emerged as a versatile tool for the interaction assay between small organic molecules and their protein receptors. We report herein the proof-of-principle of a terminal protection assay of small-molecule-linked DNA. This assay is based on our new finding that single-stranded DNA (ssDNA) terminally tethered to a small molecule is protected from the degradation by exonuclease I (Exo I) when the small molecule moiety is bound to its protein target. This finding translates the binding of small molecules to proteins into the presence of a specific DNA sequence, which enables us to probe the interaction between small organic molecules and their protein targets using various DNA sequence amplification and detection technologies. On the basis of selective assembly of single-walled carbon nanotubes (SWNTs) with surface-tethered small-molecule-linked ssDNA not protected by protein binding, a novel electrochemical strategy for terminal protection assay has been developed. Through detecting the redox signal mediated by SWNT assembly on a 16-mercaptohexadecanoic acid-blocked electrode, this strategy is able to ensure substantial signal amplification and a low background current. This strategy is demonstrated for quantitative analysis of the interaction of folate with a tumor biomarker of folate receptor (FR), and a detection limit of 3 pM FR is readily achieved with desirable specificity and sensitivity, indicating that the terminal protection assay can offer a promising platform for small molecule-protein interaction studies.

摘要

小分子连接的DNA已成为一种通用工具,用于小分子有机化合物与其蛋白质受体之间的相互作用检测。我们在此报告小分子连接的DNA末端保护检测的原理验证。该检测基于我们的新发现,即当小分子部分与其蛋白质靶标结合时,末端连接到小分子的单链DNA(ssDNA)可免受核酸外切酶I(Exo I)的降解。这一发现将小分子与蛋白质的结合转化为特定DNA序列的存在,这使我们能够使用各种DNA序列扩增和检测技术来探测小分子有机化合物与其蛋白质靶标之间的相互作用。基于单壁碳纳米管(SWNTs)与未受蛋白质结合保护的表面连接小分子连接的ssDNA的选择性组装,开发了一种用于末端保护检测的新型电化学策略。通过检测16-巯基十六烷酸封闭电极上由SWNT组装介导的氧化还原信号,该策略能够确保显著的信号放大和低背景电流。该策略用于叶酸与叶酸受体(FR)肿瘤生物标志物相互作用的定量分析,以理想的特异性和灵敏度轻松实现了3 pM FR的检测限,表明末端保护检测可为小分子-蛋白质相互作用研究提供一个有前景的平台。

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