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基于分子结合的分裂适体与 γ-环糊精的组装:适体生物传感器的灵敏激基缔合物信号方法。

Molecule-binding dependent assembly of split aptamer and γ-cyclodextrin: a sensitive excimer signaling approach for aptamer biosensors.

机构信息

State Key Laboratory of Chemo/Biosensing and Chemometrics, College of Chemistry and Chemical Engineering, Hunan University, Changsha 410082, PR China; Hubei Key Laboratory of Mine Environmental Pollution Control & Remediation, Environmental Science and Engineering College, Hubei Polytechnic University, Huangshi 435003, PR China.

出版信息

Anal Chim Acta. 2013 Oct 17;799:44-50. doi: 10.1016/j.aca.2013.08.012. Epub 2013 Sep 5.

Abstract

A highly sensitive and selective fluorescence aptamer biosensors for the determination of adenosine triphosphate (ATP) was developed. Binding of a target with splitting aptamers labeled with pyrene molecules form stable pyrene dimer in the γ-cyclodextrin (γ-CD) cavity, yielding a strong excimer emission. We have found that inclusion of pyrene dimer in γ-cyclodextrin cavity not only exhibits additive increases in quantum yield and emission lifetime of the excimer, but also facilitates target-induced fusion of the splitting aptamers to form the aptamer/target complex. As proof-of-principle, the approach was applied to fluorescence detection of adenosine triphosphate. With an anti-ATP aptamer, the approach exhibits excimer fluorescence response toward ATP with a maximum signal-to-background ratio of 32.1 and remarkably low detection limit of 80 nM ATP in buffer solution. Moreover, due to the additive fluorescence lifetime of excimer induced by γ-cyclodextrin, time-resolved measurements could be conveniently used to detect as low as 0.5 μM ATP in blood serum quantitatively.

摘要

一种用于检测三磷酸腺苷(ATP)的高灵敏和选择性荧光适体生物传感器被开发出来。带吡咯分子标记的靶标与分裂适体的结合在γ-环糊精(γ-CD)腔中形成稳定的吡咯二聚体,产生强的激基缔合物发射。我们发现,将吡咯二聚体包含在γ-环糊精腔中不仅表现出量子产率和激基缔合物发射寿命的附加增加,而且还促进了分裂适体的靶标诱导融合,形成适体/靶标复合物。作为原理验证,该方法被应用于荧光检测三磷酸腺苷。使用抗-ATP 适体,该方法对 ATP 表现出激基缔合物荧光响应,在缓冲溶液中的最大信号与背景比为 32.1,检测限低至 80 nM ATP。此外,由于 γ-环糊精诱导的激基缔合物的附加荧光寿命,时间分辨测量可以方便地用于定量检测低至 0.5 μM 的血清中的 ATP。

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