Automated forward and reverse ratcheting of DNA in a nanopore at 5-Å precision

被引:474
作者
Cherf, Gerald M. [1 ]
Lieberman, Kate R. [1 ]
Rashid, Hytham [1 ]
Lam, Christopher E. [1 ]
Karplus, Kevin [1 ]
Akeson, Mark [1 ]
机构
[1] Univ Calif Santa Cruz, Dept Biomol Engn, Nanopore Grp, Santa Cruz, CA 95064 USA
关键词
POLYNUCLEOTIDE MOLECULES; POLYMERASE COMPLEXES; ELECTRONIC CONTROL; REPLICATION; BINDING; PROTEIN; DISCRIMINATION; PORE;
D O I
10.1038/nbt.2147
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
An emerging DNA sequencing technique uses protein or solid-state pores to analyze individual strands as they are driven in single-file order past a nanoscale sensor(1-3). However, uncontrolled electrophoresis of DNA through these nanopores is too fast for accurate base reads(4). Here, we describe forward and reverse ratcheting of DNA templates through the a-hemolysin nanopore controlled by phi29 DNA polymerase without the need for active voltage control. DNA strands were ratcheted through the pore at median rates of 2.5-40 nucleotides per second and were examined at one nucleotide spatial precision in real time. Up to 500 molecules were processed at similar to 130 molecules per hour through one pore. The probability of a registry error (an insertion or deletion) at individual positions during one pass along the template strand ranged from 10% to 24.5% without optimization. This strategy facilitates multiple reads of individual strands and is transferable to other nanopore devices for implementation of DNA sequence analysis.
引用
收藏
页码:344 / 348
页数:5
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