基于 G-四联体/硫堇 T 复合物的无标记和切口酶辅助荧光信号放大用于 RNase H 的测定。

Label-free and nicking enzyme-assisted fluorescence signal amplification for RNase H determination based on a G-quadruplexe/thioflavin T complex.

机构信息

School of Life Sciences, Central South University, Changsha 410013, China.

出版信息

Talanta. 2018 May 15;182:142-147. doi: 10.1016/j.talanta.2018.01.075. Epub 2018 Jan 31.

DOI:10.1016/j.talanta.2018.01.075

Abstract

In this paper, we describe a novel, label-free and nicking enzyme-assisted fluorescence signal amplification strategy that demonstrates to be cost efficient, sensitive, and unique for assaying the RNase H activity and inhibition based on G-quadruplex formation using a thioflavin T (ThT) dye. This novel assay method is able to detect RNase H with a detection limit of 0.03 U /mL and further exhibits a good linearity R = 0.9923 at a concentration range of 0.03-1 U/mL under optimized conditions. Moreover, the inhibition effect of gentamycin on the RNase H activity is also studied. This strategy provides a potential tool for the biochemical enzyme analysis and inhibitor screening.

摘要

在本文中，我们描述了一种新颖的、无需标记且依赖核酸内切酶的荧光信号放大策略，该策略基于 G-四链体形成，使用噻唑橙（ThT）染料，显示出在测定 RNase H 活性和抑制方面具有成本效益高、灵敏度高和独特性。该新型测定方法能够检测到 RNase H 的检测限为 0.03 U / mL，并且在优化条件下，浓度范围为 0.03-1 U / mL 时具有良好的线性关系 R = 0.9923。此外，还研究了庆大霉素对 RNase H 活性的抑制作用。该策略为生化酶分析和抑制剂筛选提供了一种潜在的工具。

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基于 G-四联体/硫堇 T 复合物的无标记和切口酶辅助荧光信号放大用于 RNase H 的测定。

Label-free and nicking enzyme-assisted fluorescence signal amplification for RNase H determination based on a G-quadruplexe/thioflavin T complex.

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