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Direct and single-molecule visualization of the solution-state structures of G-hairpin and G-triplex intermediates.直接和单分子可视化 G-发夹和 G-三链体中间体在溶液状态下的结构。
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Base-excision repair activity of uracil-DNA glycosylase monitored using the latch zone of α-hemolysin.使用α-hemolysin 的闩锁区监测尿嘧啶-DNA 糖基化酶的碱基切除修复活性。
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Nanopore force spectroscopy of aptamer-ligand complexes.适体-配体复合物的纳米孔力谱学。
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Interactions of the human telomere sequence with the nanocavity of the α-hemolysin ion channel reveal structure-dependent electrical signatures for hybrid folds.人类端粒序列与α-溶血素离子通道纳米腔的相互作用揭示了混合折叠的结构依赖性电信号特征。
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Recent trends in nanopores for biotechnology.纳米孔在生物技术中的最新趋势。
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Populated intermediates in the thermal unfolding of the human telomeric quadruplex.人类端粒四链体热解折叠中的填充中间体。
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Crown ether-electrolyte interactions permit nanopore detection of individual DNA abasic sites in single molecules.冠醚-电解质相互作用允许在单个分子中单碱基错配的单个 DNA 碱基的纳米孔检测。
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蛋白质纳米腔内人端粒序列G-四链体折叠的单分子研究

Single-molecule investigation of G-quadruplex folds of the human telomere sequence in a protein nanocavity.

作者信息

An Na, Fleming Aaron M, Middleton Eric G, Burrows Cynthia J

机构信息

Department of Chemistry, University of Utah, Salt Lake City, UT 84112.

Department of Chemistry, University of Utah, Salt Lake City, UT 84112

出版信息

Proc Natl Acad Sci U S A. 2014 Oct 7;111(40):14325-31. doi: 10.1073/pnas.1415944111. Epub 2014 Sep 15.

DOI:10.1073/pnas.1415944111
PMID:25225404
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4209999/
Abstract

Human telomeric DNA consists of tandem repeats of the sequence 5'-TTAGGG-3' that can fold into various G-quadruplexes, including the hybrid, basket, and propeller folds. In this report, we demonstrate use of the α-hemolysin ion channel to analyze these subtle topological changes at a nanometer scale by providing structure-dependent electrical signatures through DNA-protein interactions. Whereas the dimensions of hybrid and basket folds allowed them to enter the protein vestibule, the propeller fold exceeds the size of the latch region, producing only brief collisions. After attaching a 25-mer poly-2'-deoxyadenosine extension to these structures, unraveling kinetics also were evaluated. Both the locations where the unfolding processes occur and the molecular shapes of the G-quadruplexes play important roles in determining their unfolding profiles. These results provide insights into the application of α-hemolysin as a molecular sieve to differentiate nanostructures as well as the potential technical hurdles DNA secondary structures may present to nanopore technology.

摘要

人类端粒DNA由5'-TTAGGG-3'序列的串联重复组成,该序列可折叠成各种G-四链体,包括杂合、篮状和螺旋桨状折叠。在本报告中,我们展示了利用α-溶血素离子通道,通过DNA-蛋白质相互作用提供依赖于结构的电信号,在纳米尺度上分析这些细微的拓扑变化。杂合和篮状折叠的尺寸允许它们进入蛋白质前庭,而螺旋桨状折叠超过了闩锁区域的大小,只产生短暂的碰撞。在这些结构上连接一个25聚体的聚2'-脱氧腺苷延伸后,还评估了解旋动力学。解旋过程发生的位置和G-四链体的分子形状在决定它们的解旋图谱中都起着重要作用。这些结果为α-溶血素作为分子筛区分纳米结构的应用以及DNA二级结构可能给纳米孔技术带来的潜在技术障碍提供了见解。