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本文引用的文献

1
Mechanism of one-way traffic of hexameric phi29 DNA packaging motor with four electropositive relaying layers facilitating antiparallel revolution.六聚体 phi29 DNA 包装马达单向运输的机制,四个正电荷中继层促进了反平行旋转。
ACS Nano. 2013 May 28;7(5):4082-92. doi: 10.1021/nn4002775. Epub 2013 Mar 26.
2
Solid-State and Biological Nanopore for Real-Time Sensing of Single Chemical and Sequencing of DNA.用于单分子化学实时传感和DNA测序的固态及生物纳米孔
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3
Incorporation of a viral DNA-packaging motor channel in lipid bilayers for real-time, single-molecule sensing of chemicals and double-stranded DNA.将病毒 DNA 包装马达通道整合到脂质双层中,用于实时、单分子检测化学物质和双链 DNA。
Nat Protoc. 2013 Feb;8(2):373-92. doi: 10.1038/nprot.2013.001. Epub 2013 Jan 24.
4
Formation of lipid bilayers inside microfluidic channel array for monitoring membrane-embedded nanopores of phi29 DNA packaging nanomotor.在微流控通道阵列内形成脂质双层以监测 phi29 DNA 包装纳米马达的膜嵌入纳米孔。
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"Push through one-way valve" mechanism of viral DNA packaging.“推动单向阀”机制的病毒 DNA 包装。
Adv Virus Res. 2012;83:415-65. doi: 10.1016/B978-0-12-394438-2.00009-8.
6
Real-time sensing and discrimination of single chemicals using the channel of phi29 DNA packaging nanomotor.利用 phi29 DNA 包装纳米马达通道实时感应和区分单个化学物质。
ACS Nano. 2012 Apr 24;6(4):3251-61. doi: 10.1021/nn3001615. Epub 2012 Apr 9.
7
Stochastic sensing of proteins with receptor-modified solid-state nanopores.用受体修饰的固态纳米孔对蛋白质进行随机感应。
Nat Nanotechnol. 2012 Mar 11;7(4):257-63. doi: 10.1038/nnano.2012.24.
8
Role of channel lysines and the "push through a one-way valve" mechanism of the viral DNA packaging motor.病毒 DNA 包装马达的通道赖氨酸作用和“推过单向阀”机制。
Biophys J. 2012 Jan 4;102(1):127-35. doi: 10.1016/j.bpj.2011.11.4013. Epub 2012 Jan 3.
9
Nanopore sensors for nucleic acid analysis.纳米孔传感器用于核酸分析。
Nat Nanotechnol. 2011 Sep 18;6(10):615-24. doi: 10.1038/nnano.2011.129.
10
Thermodynamically stable RNA three-way junction for constructing multifunctional nanoparticles for delivery of therapeutics.用于构建多功能纳米粒子以递送电疗药物的热力学稳定 RNA 三链结。
Nat Nanotechnol. 2011 Sep 11;6(10):658-67. doi: 10.1038/nnano.2011.105.

Phi29 噬菌体 DNA 包装纳米马达的通道尺寸转换用于单链和双链核酸的区分。

Channel size conversion of Phi29 DNA-packaging nanomotor for discrimination of single- and double-stranded nucleic acids.

机构信息

Nanobiotechnology Center, Department of Pharmaceutical Sciences, University of Kentucky, Lexington, Kentucky 40536, United States.

出版信息

ACS Nano. 2013 Apr 23;7(4):3315-23. doi: 10.1021/nn400020z. Epub 2013 Mar 25.

DOI:10.1021/nn400020z
PMID:23488809
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3663147/
Abstract

Nanopores have been utilized to detect the conformation and dynamics of polymers, including DNA and RNA. Biological pores are extremely reproducible at the atomic level with uniform channel sizes. The channel of the bacterial virus phi29 DNA-packaging motor is a natural conduit for the transportation of double-stranded DNA (dsDNA) and has the largest diameter among the well-studied biological channels. The larger channel facilitates translocation of dsDNA and offers more space for further channel modification and conjugation. Interestingly, the relatively large wild-type channel, which translocates dsDNA, cannot detect single-stranded nucleic acids (ssDNA or ssRNA) under the current experimental conditions. Herein, we reengineered this motor channel by removing the internal loop segment of the channel. The modification resulted in two classes of channels. One class was the same size as the wild-type channel, while the other class had a cross-sectional area about 60% of the wild-type. This smaller channel was able to detect the real-time translocation of single-stranded nucleic acids at single-molecule level. While the wild-type connector exhibited a one-way traffic property with respect to dsDNA translocation, the loop-deleted connector was able to translocate ssDNA and ssRNA with equal competencies from both termini. This finding of size alterations in reengineered motor channels expands the potential application of the phi29 DNA-packaging motor in nanomedicine, nanobiotechnology, and high-throughput single-pore DNA sequencing.

摘要

纳米孔已被用于检测聚合物的构象和动力学,包括 DNA 和 RNA。生物孔在原子水平上具有极高的重现性,通道尺寸均匀。细菌病毒 phi29 DNA 包装马达的通道是双链 DNA(dsDNA)运输的天然通道,其直径在研究充分的生物通道中是最大的。较大的通道有利于 dsDNA 的易位,并为进一步的通道修饰和连接提供了更多空间。有趣的是,相对较大的野生型通道虽然可以转运 dsDNA,但在当前的实验条件下,无法检测单链核酸(ssDNA 或 ssRNA)。在此,我们通过去除通道内部环段对该马达通道进行了重新设计。这种修饰产生了两类通道。一类与野生型通道大小相同,而另一类的横截面积约为野生型的 60%。这个较小的通道能够在单分子水平上实时检测单链核酸的易位。虽然野生型接头在 dsDNA 易位方面表现出单向交通特性,但环缺失接头能够以同等的能力从两端转运 ssDNA 和 ssRNA。这种在重新设计的马达通道中改变大小的发现,扩展了 phi29 DNA 包装马达在纳米医学、纳米生物技术和高通量单孔 DNA 测序中的潜在应用。