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基于外切核酸酶 I 辅助的铁掺杂多孔碳-氮掺杂石墨烯量子点双磁分离荧光法检测赭曲霉毒素 A

Exonuclease I-assisted fluorescent method for ochratoxin A detection using iron-doped porous carbon, nitrogen-doped graphene quantum dots, and double magnetic separation.

机构信息

College of Food and Biological Engineering, Jiangsu University, Zhenjiang, 212013, China.

出版信息

Anal Bioanal Chem. 2019 Apr;411(11):2405-2414. doi: 10.1007/s00216-019-01684-7. Epub 2019 Mar 4.

Abstract

In this paper, a fluorescent method was developed for ochratoxin A (OTA) detection that uses iron-doped porous carbon (MPC) and aptamer-functionalized nitrogen-doped graphene quantum dots (NGQDs-Apt) as probes. In this method, the adsorbance of the NGQDs-Apt on the MPC due to a π-π interaction between the aptamer and the MPC results in the quenching of the fluorescence of the NGQDs-Apt. However, since OTA interacts strongly with the aptamer, the presence of OTA leads to the detachment of the NGQDs-Apt from the MPC, resulting in the resumption of fluorescence from the NGQDs-Apt. When exonuclease I (Exo I) is also added to the solution, this exonuclease specifically digests the aptamer, leading to the release of the OTA back into the solution. This free OTA then interacts with another MPC-NGQDs-Apt system, inducing the release of more NGQDs into the solution, which enhances the fluorescent intensity compared to that of the system with no Exo I. Utilizing this behavior of OTA in the presence of NGQDs-Apt, it was possible to detect concentrations of OTA ranging from 10 to 5000 nM, with a limit of detection of 2.28 nM. Our method was tested by applying it to the detection of OTA in wheat and corn samples. This method has four advantages: (1) the magnetic porous carbon is easy to prepare, its porosity enhances its loading capacity for NGQDs, it highly efficiently quenches the fluorescence of the NGQDs, and its magnetic properties facilitate the separation of the MPC from other species in solution; (2) applying double magnetic separation decreases the background signal; (3) Exo I digests the free aptamer effectively, which allows the resulting free OTA to induce the release of more NGQDs-Apt, ultimately enhancing the fluorescent signal; and (4) the proposed method presented high sensitivity and a wide linear detection range. This method may prove helpful in food safety analysis and new biosensor development (achieved by using different aptamer sequences to that used in the present work). Graphical abstract Exonuclease I (Exo I)-assisted fluorescent method for ochratoxin A (OTA) detection using magnetic porous carbon (MPC), nitrogen-doped graphene quantum dots (NGQDs), and double magnetic separation.

摘要

本文开发了一种利用铁掺杂多孔碳(MPC)和适配体功能化氮掺杂石墨烯量子点(NGQDs-Apt)作为探针检测赭曲霉毒素 A(OTA)的荧光方法。在该方法中,由于适配体与 MPC 之间的π-π相互作用,NGQDs-Apt 在 MPC 上的吸附导致 NGQDs-Apt 的荧光猝灭。然而,由于 OTA 与适配体强烈相互作用,OTA 的存在导致 NGQDs-Apt 从 MPC 上脱离,从而恢复 NGQDs-Apt 的荧光。当外切酶 I(Exo I)也被添加到溶液中时,这种外切酶特异性地消化适配体,导致 OTA 被释放回溶液中。然后,这种游离的 OTA 与另一个 MPC-NGQDs-Apt 系统相互作用,导致更多的 NGQDs 被释放到溶液中,与没有 Exo I 的系统相比,荧光强度增强。利用 OTA 在 NGQDs-Apt 存在下的这种行为,可以检测到 10 到 5000 nM 的 OTA 浓度,检测限为 2.28 nM。我们的方法通过将其应用于小麦和玉米样品中 OTA 的检测来进行测试。该方法具有四个优点:(1) 磁性多孔碳易于制备,其多孔性增强了其对 NGQDs 的负载能力,高效地猝灭了 NGQDs 的荧光,其磁性有利于 MPC 从溶液中的其他物质中分离;(2) 应用双重磁分离降低了背景信号;(3) Exo I 有效地消化游离的适配体,使游离的 OTA 诱导更多的 NGQDs-Apt 释放,最终增强荧光信号;(4) 所提出的方法具有高灵敏度和宽线性检测范围。该方法可能有助于食品安全分析和新生物传感器的开发(通过使用与本工作中使用的不同的适配体序列来实现)。

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