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用于检测 ATP 的荧光 G-四链体适体传感器的开启型和比率型检测方法的比较。

Comparison of turn-on and ratiometric fluorescent G-quadruplex aptasensor approaches for the detection of ATP.

机构信息

Department of Biotechnology, VIT Vellore, Vellore, Tamil Nadu, 632 104, India.

Department of Chemistry, Carleton University, 1125 Colonel By Drive, Ottawa, ON, K1S 5B6, Canada.

出版信息

Anal Bioanal Chem. 2019 Mar;411(7):1319-1330. doi: 10.1007/s00216-018-1484-x. Epub 2019 Jan 5.

DOI:10.1007/s00216-018-1484-x
PMID:30612178
Abstract

Two fluorescent aptasensor methods were developed for the detection of ATP in biochemical systems. The first method consisted of a label-free fluorescent "turn-on" approach using a guanine-rich ATP aptamer sequence and the DNA-binding agent berberine complex. In the presence of ATP, the ATP preferentially binds with its aptamer and conformationally changes into a G-quadruplex structure. The association of berberine with the G-quadruplex results in the enhancement of the fluorescence signal of the former. The detection limit of ATP was found to be 3.5 μM. Fluorescence, circular dichroism and melting temperature (T) experiments were carried out to confirm the binding specificity and structural changes. The second method employs the ratiometric fluorescent approach based on the Forster resonance energy transfer (FRET) for the detection of ATP using berberine along with a quencher (AuNRs, AgNPs) and a fluorophore (red quantum dots (RQDs), carbon dots (CDs)) labeled at 5' and 3' termini of the ATP-binding aptamer sequence. Upon addition of ATP and berberine, ATP specifically binds with its aptamer leading to the formation of G-quadruplex, and similarly, berberine also binds to the G-quadruplex. This leads to an enhancement of fluorescence of berberine while that of RQD and CDs were significantly quenched via FRET. The respective detection limits calculated were 3.6 μM and 3.8 μM, indicating these fluorescent aptasensor methods may be used for a wide variety of small molecules. Graphical abstract.

摘要

两种荧光适体传感器方法被开发用于生化系统中 ATP 的检测。第一种方法是使用富含鸟嘌呤的 ATP 适体序列和 DNA 结合剂小檗碱复合物的无标记荧光“开启”方法。在 ATP 存在的情况下,ATP 优先与其适体结合,并构象变为 G-四链体结构。小檗碱与 G-四链体的结合导致前者的荧光信号增强。发现 ATP 的检测限为 3.5 μM。进行了荧光、圆二色性和熔点 (T) 实验以确认结合特异性和结构变化。第二种方法采用比率荧光法,基于福斯特共振能量转移 (FRET),使用小檗碱以及淬灭剂 (AuNRs、AgNPs) 和标记在 ATP 结合适体序列 5' 和 3' 末端的荧光团 (红色量子点 (RQDs)、碳点 (CDs)) 来检测 ATP。加入 ATP 和小檗碱后,ATP 特异性地与其适体结合,导致 G-四链体的形成,类似地,小檗碱也与 G-四链体结合。这导致小檗碱的荧光增强,而 RQD 和 CDs 的荧光通过 FRET 显著猝灭。计算出的各自检测限分别为 3.6 μM 和 3.8 μM,表明这些荧光适体传感器方法可用于广泛的小分子。

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