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基于数字编码硅基微球和 RCA 级联扩增的高灵敏、多重 miRNA 分析。

Highly sensitive and multiplexed miRNA analysis based on digitally encoded silica microparticles coupled with RCA-based cascade amplification.

机构信息

Key Laboratory for Nano-Bio Interface Research, Nano-Bio-Chem Centre, Suzhou Institute of Nano-Tech and Nano-Bionics, Chinese Academy of Sciences, Suzhou, 215123, China.

出版信息

Analyst. 2018 Oct 22;143(21):5137-5144. doi: 10.1039/c8an01393d.

Abstract

Currently, miRNA analysis is significant for understanding miRNA regulation networks and clinical diagnostics and therapy. Analytical strategies feasible for multiplex miRNA-sensitive analysis are still in high demand. Herein, we propose a novel strategy for miRNA analysis by coupling cascade amplification with digitally encoded silica microparticles. The microparticles are precisely fabricated in a digital form through a one-step deposition strategy and are highly efficient for multiplex analysis. The cascade amplification composed of RCA and nicking-assisted strand-displacement amplification (SDA) exhibits high amplification efficiency and requires no complicated sequence design, thus improving the compatibility with base-stacking hybridization on our microparticles. Parallel and sensitive analyses for let-7a and miR-21 in one pot without mutual interference have been achieved with both high sensitivity (LOD, ∼0.5 fM) and wide dynamic range (10 pM-1 fM). Moreover, our strategy exhibits high specificity for miRNAs of homologous sequence and good anti-interference ability in a complex sample matrix. Considering that there are up to 128 (27) kinds of microparticles available, our strategy can be applied for dozens of miRNA-sensitive analyses in one pot, and it has great potential for miRNA signature analysis as well as widespread clinical applications.

摘要

目前,miRNA 分析对于理解 miRNA 调控网络和临床诊断与治疗具有重要意义。因此,人们仍然迫切需要能够对多种 miRNA 进行敏感分析的分析策略。本文提出了一种通过级联扩增与数字编码硅基微球偶联进行 miRNA 分析的新策略。通过一步沉积策略精确地以数字形式制备微球,其具有高效的多重分析能力。由 RCA 和缺口辅助链置换扩增(SDA)组成的级联扩增具有高扩增效率,且无需复杂的序列设计,从而提高了与我们微球上碱基堆积杂交的兼容性。通过一锅法实现了 let-7a 和 miR-21 的平行和敏感分析,且具有高灵敏度(LOD,约 0.5 fM)和宽动态范围(10 pM-1 fM)。此外,我们的策略对同源序列的 miRNA 具有高特异性,且在复杂样本基质中具有良好的抗干扰能力。考虑到多达 128(27)种微球可供使用,我们的策略可以在一个反应体系中进行数十种 miRNA 敏感分析,因此其在 miRNA 特征分析以及广泛的临床应用中具有很大的潜力。

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