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本文引用的文献

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High-throughput real-time quantitative reverse transcription PCR.高通量实时定量逆转录PCR
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2
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Nucleic Acids Res. 2008 Mar;36(5):1532-41. doi: 10.1093/nar/gkm1017. Epub 2008 Jan 21.
3
A single-molecule nanopore device detects DNA polymerase activity with single-nucleotide resolution.一种单分子纳米孔装置能够以单核苷酸分辨率检测DNA聚合酶活性。
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Detection of DNA sequences using an alternating electric field in a nanopore capacitor.利用纳米孔电容器中的交变电场检测DNA序列。
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Exploring transmembrane transport through alpha-hemolysin with grid-steered molecular dynamics.利用网格导向分子动力学探索通过α-溶血素的跨膜运输。
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Progress toward ultrafast DNA sequencing using solid-state nanopores.利用固态纳米孔实现超快速DNA测序的进展。
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Detecting SNPs using a synthetic nanopore.使用合成纳米孔检测单核苷酸多态性。
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8
Single-molecule electrophoresis of beta-hairpin peptides by electrical recordings and Langevin dynamics simulations.通过电记录和朗之万动力学模拟对β-发夹肽进行单分子电泳
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发夹DNA通过合成纳米孔的微观力学

Microscopic mechanics of hairpin DNA translocation through synthetic nanopores.

作者信息

Comer Jeffrey, Dimitrov Valentin, Zhao Qian, Timp Gregory, Aksimentiev Aleksei

机构信息

Department of Physics, University of Illinois, Urbana, Illinois, USA.

出版信息

Biophys J. 2009 Jan;96(2):593-608. doi: 10.1016/j.bpj.2008.09.023.

DOI:10.1016/j.bpj.2008.09.023
PMID:19167307
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2716687/
Abstract

Nanoscale pores have proved useful as a means to assay DNA and are actively being developed as the basis of genome sequencing methods. Hairpin DNA (hpDNA), having both double-helical and overhanging coil portions, can be trapped in a nanopore, giving ample time to execute a sequence measurement. In this article, we provide a detailed account of hpDNA interaction with a synthetic nanopore obtained through extensive all-atom molecular dynamics simulations. For synthetic pores with minimum diameters from 1.3 to 2.2 nm, we find that hpDNA can translocate by three modes: unzipping of the double helix and--in two distinct orientations--stretching/distortion of the double helix. Furthermore, each of these modes can be selected by an appropriate choice of the pore size and voltage applied transverse to the membrane. We demonstrate that the presence of hpDNA can dramatically alter the distribution of ions within the pore, substantially affecting the ionic current through it. In experiments and simulations, the ionic current relative to that in the absence of DNA can drop below 10% and rise beyond 200%. Simulations associate the former with the double helix occupying the constriction and the latter with accumulation of DNA that has passed through the constriction.

摘要

纳米级孔隙已被证明可作为检测DNA的一种手段,并且正积极被开发作为基因组测序方法的基础。发夹DNA(hpDNA)同时具有双螺旋部分和突出的卷曲部分,可被困在纳米孔中,从而有足够时间进行序列测量。在本文中,我们通过广泛的全原子分子动力学模拟,详细阐述了hpDNA与合成纳米孔的相互作用。对于最小直径为1.3至2.2nm的合成孔,我们发现hpDNA可以通过三种模式进行转运:双螺旋解链以及——在两种不同取向下——双螺旋的拉伸/变形。此外,这些模式中的每一种都可以通过适当选择孔径和施加于膜的横向电压来选择。我们证明,hpDNA的存在可以显著改变孔内离子的分布,从而极大地影响通过它的离子电流。在实验和模拟中,相对于不存在DNA时的离子电流,离子电流可降至10%以下,也可升至200%以上。模拟将前者与占据收缩处的双螺旋相关联,而将后者与通过收缩处的DNA积累相关联。