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在双纳米孔设备中控制 DNA 拔河比赛。

Controlling DNA Tug-of-War in a Dual Nanopore Device.

机构信息

Ontera, Inc., Santa Cruz, CA, 95060, USA.

Department of Physics, McGill University, Montreal, QC, H3A 2T8, Canada.

出版信息

Small. 2019 Jul;15(30):e1901704. doi: 10.1002/smll.201901704. Epub 2019 Jun 13.

DOI:10.1002/smll.201901704
PMID:31192541
Abstract

Methods for reducing and directly controlling the speed of DNA through a nanopore are needed to enhance sensing performance for direct strand sequencing and detection/mapping of sequence-specific features. A method is created for reducing and controlling the speed of DNA that uses two independently controllable nanopores operated with an active control logic. The pores are positioned sufficiently close to permit cocapture of a single DNA by both pores. Once cocapture occurs, control logic turns on constant competing voltages at the pores leading to a "tug-of-war" whereby opposing forces are applied to regions of the molecules threading through the pores. These forces exert both conformational and speed control over the cocaptured molecule, removing folds and reducing the translocation rate. When the voltages are tuned so that the electrophoretic force applied to both pores comes into balance, the life time of the tug-of-war state is limited purely by diffusive sliding of the DNA between the pores. A tug-of-war state is produced on 76.8% of molecules that are captured with a maximum two-order of magnitude increase in average pore translocation time relative to the average time for single-pore translocation. Moreover, the translocation slow-down is quantified as a function of voltage tuning and it is shown that the slow-down is well described by a first passage analysis for a 1D subdiffusive process. The ionic current of each nanopore provides an independent sensor that synchronously measures a different region of the same molecule, enabling sequential detection of physical labels, such as monostreptavidin tags. With advances in devices and control logic, future dual-pore applications include genome mapping and enzyme-free sequencing.

摘要

需要开发用于降低和直接控制 DNA 通过纳米孔速度的方法,以提高直接链测序和检测/定位序列特异性特征的传感性能。本文提出了一种用于降低和控制 DNA 速度的方法,该方法使用两个独立可控的纳米孔,并采用主动控制逻辑进行操作。这些孔被定位得足够近,以便两个孔都能同时捕获单链 DNA。一旦发生共捕获,控制逻辑会在两个孔上开启恒定的竞争电压,导致“拔河”现象,从而将相反的力施加到穿过孔的分子的区域。这些力对共捕获的分子施加构象和速度控制,去除折叠并降低迁移率。当电压被调谐使得施加到两个孔的电泳力达到平衡时,拔河状态的寿命仅受 DNA 在孔之间扩散滑动的限制。在捕获的分子中有 76.8%产生拔河状态,相对于单孔迁移的平均时间,平均孔迁移时间增加了两个数量级。此外,还对电压调谐的慢化进行了量化,并表明慢化可以通过一维亚扩散过程的首次通过分析来很好地描述。每个纳米孔的离子电流提供了一个独立的传感器,同步测量同一分子的不同区域,从而能够对物理标记(如单链亲和素标签)进行顺序检测。随着设备和控制逻辑的进步,未来的双孔应用包括基因组作图和无酶测序。

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