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通过控制计数实现纳米孔的精确 DNA 浓度测量。

Precise DNA Concentration Measurements with Nanopores by Controlled Counting.

机构信息

Department of Physics , University of Ottawa , 150 Louis-Pasteur , Ottawa , Ontario , Canada K1N 6N5.

出版信息

Anal Chem. 2019 Oct 1;91(19):12228-12237. doi: 10.1021/acs.analchem.9b01900. Epub 2019 Sep 10.

DOI:10.1021/acs.analchem.9b01900
PMID:31438671
Abstract

Using a solid-state nanopore to measure the concentration of clinically relevant target analytes, such as proteins or specific DNA sequences, is a major goal of nanopore research. This is usually achieved by measuring the capture rate of the target analyte through the pore. However, progress is hindered by sources of systematic error that are beyond the level of control currently achievable with state-of-the-art nanofabrication techniques. In this work, we show that the capture rate process of solid-state nanopores is subject to significant sources of variability, both within individual nanopores over time and between different nanopores of nominally identical size, which are absent from theoretical electrophoretic capture models. We experimentally reveal that these fluctuations are inherent to the nanopore itself and make nanopore-based molecular concentration determination insufficiently precise to meet the standards of most applications. In this work, we present a simple method by which to reduce this variability, increasing the reliability, accuracy, and precision of single-molecule nanopore-based concentration measurements. We demonstrate controlled counting, a concentration measurement technique, which involves measuring the simultaneous capture rates of a mixture of both the target molecule and an internal calibrator of precisely known concentration. Using this method on linear DNA fragments, we show empirically that the requirements for precisely controlling the nanopore properties, including its size, height, geometry, and surface charge density or distribution, are removed while allowing for higher-precision measurements. The quantitative tools presented herein will greatly improve the utility of solid-state nanopores as sensors of target biomolecule concentration.

摘要

利用固态纳米孔来测量具有临床相关性的目标分析物(如蛋白质或特定 DNA 序列)的浓度,是纳米孔研究的主要目标。这通常是通过测量目标分析物通过孔的捕获率来实现的。然而,由于目前的纳米制造技术还无法控制的系统误差来源,这一进展受到了阻碍。在这项工作中,我们表明,固态纳米孔的捕获率过程受到显著的可变性的影响,这些可变性既存在于单个纳米孔随时间的变化中,也存在于名义上相同尺寸的不同纳米孔之间,而这些变化在理论电泳捕获模型中是不存在的。我们通过实验揭示了这些波动是纳米孔本身固有的,使得基于纳米孔的分子浓度测定不够精确,无法满足大多数应用的标准。在这项工作中,我们提出了一种简单的方法来降低这种可变性,从而提高基于单分子纳米孔的浓度测量的可靠性、准确性和精度。我们展示了受控计数,这是一种浓度测量技术,它涉及测量目标分子和精确已知浓度的内部校准分子的同时捕获率。我们使用这种方法对线性 DNA 片段进行了实证研究,结果表明,精确控制纳米孔特性(包括其尺寸、高度、几何形状以及表面电荷密度或分布)的要求被消除了,同时允许进行更高精度的测量。本文提出的定量工具将极大地提高固态纳米孔作为目标生物分子浓度传感器的实用性。

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