Single-molecule measurements of synthesis by DNA polymerase with base-pair resolution

被引:73
|
作者
Christian, Thomas D. [1 ]
Romano, Louis J. [1 ]
Rueda, David [1 ]
机构
[1] Wayne State Univ, Dept Chem, Detroit, MI 48202 USA
基金
美国国家科学基金会; 美国国家卫生研究院;
关键词
Klenow Fragment; polymerase and exonuclease site; single molecule fluorescence; single nucleotide resolution; structural dynamics; I KLENOW FRAGMENT; ESCHERICHIA-COLI; KINETIC MECHANISM; STRUCTURAL BASIS; CONFORMATIONAL-CHANGE; FINGERS SUBDOMAIN; SIDE-CHAINS; IDENTIFICATION; FIDELITY; SITES;
D O I
10.1073/pnas.0908640106
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
The catalytic mechanism of DNA polymerases involves multiple steps that precede and follow the transfer of a nucleotide to the 3'-hydroxyl of the growing DNA chain. Here we report a single-molecule approach to monitor the movement of E. coli DNA polymerase I (Klenow fragment) on a DNA template during DNA synthesis with single base-pair resolution. As each nucleotide is incorporated, the single-molecule Forster resonance energy transfer intensity drops in discrete steps to values consistent with single-nucleotide incorporations. Purines and pyrimidines are incorporated with comparable rates. A mismatched primer/template junction exhibits dynamics consistent with the primer moving into the exonuclease domain, which was used to determine the fraction of primer-termini bound to the exonuclease and polymerase sites. Most interestingly, we observe a structural change after the incorporation of a correctly paired nucleotide, consistent with transient movement of the polymerase past the preinsertion site or a conformational change in the polymerase. This may represent a previously unobserved step in the mechanism of DNA synthesis that could be part of the proofreading process.
引用
收藏
页码:21109 / 21114
页数:6
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