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抗杀虫剂 DNA 适体未能识别其目标,具有声称的微摩尔离解常数。

Anti-pesticide DNA aptamers fail to recognize their targets with asserted micromolar dissociation constants.

机构信息

Univ. Grenoble Alpes, CNRS, DPM, 38000, Grenoble, France; Novaptech, 2 Allée Du Doyen Georges Brus, 33600, Pessac, France.

Univ. Grenoble Alpes, CNRS, DPM, 38000, Grenoble, France.

出版信息

Anal Chim Acta. 2021 May 15;1159:338382. doi: 10.1016/j.aca.2021.338382. Epub 2021 Mar 20.

DOI:10.1016/j.aca.2021.338382
PMID:33867041
Abstract

Herein, we originally aimed at developing fluorescence anisotropy biosensor platforms devoted to the homogeneous-phase detection of isocarbophos and phorate pesticides by using previously isolated DNA aptamers. To achieve this, two reporting approaches displaying very high generalizability features were implemented, based on either the complementary strand or the SYBR green intercalator displacement strategies. Unfortunately, none of the transduction methods led to phorate-dependent signals. Only the SYBR green displacement method provided a small output in the presence of isocarbophos, but at an analyte concentration greater than 100 μM. In order to identify the origin of such data, isothermal titration calorimetry (ITC) experiments were subsequently performed. It was shown that aptamers bind neither isocarbophos nor phorate in free solution with the claimed micromolar dissociation constants. This work puts forward some doubts about the previously described aptasensors that rely on the use of these functional DNA molecules. It also highlights the need to carefully investigate the binding capabilities of aptamers after their isolation and to include appropriate control experiments with scrambled or mutated oligonucleotides.

摘要

在此,我们最初旨在开发荧光各向异性生物传感器平台,通过使用先前分离的 DNA 适体,用于均相检测异稻瘟净和甲拌磷农药。为了实现这一目标,我们实施了两种具有高度通用性特征的报告方法,基于互补链或 SYBR 绿嵌入剂置换策略。不幸的是,没有一种转导方法导致依赖于甲拌磷的信号。只有 SYBR 绿置换法在存在异稻瘟净的情况下提供了一个小的输出,但在分析物浓度大于 100μM 时。为了确定这些数据的来源,随后进行了等温滴定量热法 (ITC) 实验。结果表明,适体在游离溶液中既不与异稻瘟净也不与甲拌磷结合,其声称的离解常数为微摩尔。这项工作对以前依赖于使用这些功能 DNA 分子的适体传感器提出了一些质疑。它还强调了需要在分离后仔细研究适体的结合能力,并包括用随机或突变寡核苷酸进行适当的对照实验。

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