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用于快速读出的小分子检测的即用型免疫传感器。

"Ready-to-use" immunosensor for the detection of small molecules with fast readout.

机构信息

College of Plant Protection, Nanjing Agricultural University, Nanjing, 210095, China; State & Local Joint Engineering Research Center of Green Pesticide Invention and Application, Nanjing, 210095, China.

Cátedra de Inmunología, Facultad de Química, Instituto de Higiene, Universidad de la República, Montevideo, 11600, Uruguay.

出版信息

Biosens Bioelectron. 2022 Apr 1;201:113968. doi: 10.1016/j.bios.2022.113968. Epub 2022 Jan 6.

Abstract

Immunoassays are commonly used methods for detection of small molecules that typically require numerous steps of the labeling between immune-recognition reagents and tracers, immobilization and recurrent washing, making them time consuming and difficult to adapt into point of care formats. Here we describe a "ready-to-use" homogeneous competitive immunosensor with an assay time of 10 min that is based exclusively on recombinant reagents. The signal is produced when the split fragments of the nano luciferase (Nluc) are brought together by the interaction of a heavy chain only variable domain (VHH) with a peptidomimetic of the target small molecule. A VHH to 2,4-dichlorophenoxyacetic acid (2,4-D) was used to isolated the peptidomimetic (NGFFEPWQVVYV) from phage display libraries using six panning conditions. Then the peptidomimetic and VHH were fused with the larger (LgN) and smaller piece (SmN) of split fragments of Nluc, respectively. In order to optimize the signal and sensitivity of the immunosensor, we explored the effects of the spacer between the peptidomimetic and LgN, the copy number of peptidomimetics, and the spacer between SmN and VHH, generating 24 combinations that allowed to conclude on their respective roles. Eventually, the developed "ready-to-use" immunosensor performed excellent signal-to-noise ratio and sensitivity, and could be applied to the detection of 2,4-D in real samples. Meanwhile, the immunosensor totally realizes labeling-free, immobilization-free and washing-free, also can be produced in a highly cost effective way.

摘要

免疫分析通常用于检测小分子,通常需要在免疫识别试剂和示踪剂之间进行多次标记、固定和反复洗涤,这使得它们耗时且难以适应即时检测的形式。在这里,我们描述了一种基于重组试剂的“即用型”均相竞争性免疫传感器,其测定时间为 10 分钟。当重链仅有可变结构域(VHH)与目标小分子的肽模拟物相互作用时,纳米荧光素酶(Nluc)的分裂片段聚集在一起,从而产生信号。使用噬菌体展示文库,我们使用六种淘选条件从噬菌体展示文库中分离出针对 2,4-二氯苯氧乙酸(2,4-D)的 VHH。然后,将肽模拟物和 VHH 分别与 Nluc 的较大片段(LgN)和较小片段(SmN)融合。为了优化免疫传感器的信号和灵敏度,我们探讨了肽模拟物和 LgN 之间的间隔、肽模拟物的拷贝数以及 SmN 和 VHH 之间的间隔对信号的影响,生成了 24 种组合,从而得出了它们各自的作用。最终,开发的“即用型”免疫传感器具有出色的信噪比和灵敏度,可用于检测真实样本中的 2,4-D。同时,该免疫传感器完全实现了无标记、无固定和无洗涤,也可以以高性价比的方式生产。

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