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构建无酶引发剂复制杂交链式反应回路用于扩增甲基转移酶评估和抑制剂测定。

Construction of an Enzyme-Free Initiator-Replicated Hybridization Chain Reaction Circuit for Amplified Methyltransferase Evaluation and Inhibitor Assay.

机构信息

College of Chemistry and Molecular Sciences, Wuhan University, Wuhan 430072, P. R. China.

出版信息

Anal Chem. 2021 Feb 2;93(4):2403-2410. doi: 10.1021/acs.analchem.0c04356. Epub 2021 Jan 4.

DOI:10.1021/acs.analchem.0c04356
PMID:33395263
Abstract

The enzyme-free nucleic acid amplification circuit, for example, hybridization chain reaction (HCR), has paved a broad avenue for evaluating various enzyme-involved biotransformations, including DNA methyltransferases (MTases). The nonenzymatic MTase-sensing platform has supplemented a versatile toolbox for monitoring aberrant methylation in intricate biological samples, yet their amplification efficiency is always constrained by the initiator-depletion paradigm. Herein, the autonomously initiator-replicated HCR (IR-HCR) was developed as a versatile amplification system for detecting MTase with ∼100-fold sensitivity of the conventional HCR system. The initiator -triggered HCR leads the assembly of a tandem DNAzyme concatemer that cleaves its substrate. This leads to the cyclic replication of a new initiator for reversely motivating the initial HCR circuit, resulting in a dramatic Förster resonance energy transfer (FRET) readout. Without M.SssI MTase, hairpin can be recognized and digested by restriction endonuclease HpaII to release initiator for stimulating a high FRET signal. While the M.SssI-methylated prohibits the HpaII-mediated cleavage of , the caged initiator fails to trigger the IR-HCR circuit. Based on a systematic investigation, the IR-HCR circuit readily achieves selective and sensitive analysis of M.SssI MTase and its inhibitors. As a general MTase-sensing platform, the IR-HCR principle was further applied to analyze another MTase (Dam) by redesigning with the Dam recognition sequence. Overall, the versatile homogeneous MTase sensing platform was achieved via an efficient and robust initiator replication amplification circuit and may have enormous potential for early disease diagnosis.

摘要

例如,无酶核酸扩增电路,如杂交链式反应 (HCR),为评估各种涉及酶的生物转化铺平了广阔的道路,包括 DNA 甲基转移酶 (MTases)。非酶 MTase 感应平台为监测复杂生物样本中的异常甲基化提供了多功能工具,但它们的扩增效率总是受到引发剂耗尽模式的限制。在此,自主引发剂复制 HCR (IR-HCR) 被开发为一种通用的扩增系统,用于检测 MTase,其灵敏度比传统 HCR 系统高约 100 倍。引发剂触发的 HCR 导致串联 DNA 酶的组装,该酶切割其底物。这导致新引发剂的循环复制,用于反向激励初始 HCR 电路,导致显著的Förster 共振能量转移 (FRET) 读出。没有 M.SssI MTase,发夹可以被限制性内切酶 HpaII 识别和消化,以释放引发剂来刺激高 FRET 信号。虽然 M.SssI 甲基化的 阻止了 HpaII 介导的 切割,但封闭的引发剂 无法触发 IR-HCR 电路。通过系统研究,IR-HCR 电路能够轻松实现对 M.SssI MTase 及其抑制剂的选择性和灵敏分析。作为一种通用的 MTase 感应平台,IR-HCR 原理通过重新设计带有 Dam 识别序列的 进一步应用于分析另一种 MTase (Dam)。总的来说,通过高效稳健的引发剂复制扩增电路实现了通用的均相 MTase 感应平台,可能在早期疾病诊断方面具有巨大的潜力。

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