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Electronic control of DNA polymerase binding and unbinding to single DNA molecules

机译:电子控制DNA聚合酶结合和解离单个DNA分子

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摘要

DNA polymerases catalyze template-dependent genome replication. The assembly of a high affinity ternary complex between these enzymes, the double strand-single strand junction of their DNA substrate, and the deoxynucleoside triphosphate (dNTP) complementary to the first template base in the polymerase active site is essential to this process. We present a single molecule method for iterative measurements of DNA-polymerase complex assembly with high temporal resolution, using active voltage control of individual DNA substrate molecules tethered noncovalently in an α-hemolysin nanopore. DNA binding states of the Klenow fragment of Escherichia coli DNA polymerase I (KF) were diagnosed based upon their ionic current signature, and reacted to with submillisecond precision to execute voltage changes that controlled exposure of the DNA substrate to KF and dNTP. Precise control of exposure times allowed measurements of DNA-KF complex assembly on a time scale that superimposed with the rate of KF binding. Hundreds of measurements were made with a single tethered DNA molecule within seconds, and dozens of molecules can be tethered within a single experiment. This approach allows statistically robust analysis of the assembly of complexes between DNA and RNA processing enzymes and their substrates at the single molecule level.
机译:DNA聚合酶催化模板依赖性基因组复制。这些酶之间的高亲和力三元复合物,其DNA底物的双链-单链连接以及与聚合酶活性位点中的第一个模板碱基互补的脱氧核苷三磷酸(dNTP)的组装对于此过程至关重要。我们提出了一种单分子方法,用于对具有高时间分辨率的DNA-聚合酶复合物组件进行迭代测量,使用对非共价结合在α-溶血素纳米孔中的单个DNA底物分子的有源电压控制。基于其离子电流特征诊断大肠杆菌DNA聚合酶I(KF)的Klenow片段的DNA结合状态,并以亚毫秒级精度反应以执行电压变化,从而控制DNA底物暴露于KF和dNTP。精确控制暴露时间可以在与KF结合速率相叠加的时间尺度上进行DNA-KF复杂装配的测量。数秒之内,用一个拴系的DNA分子即可进行数百次测量,并且可以在一个实验中拴系数十个分子。这种方法可以对单分子水平上的DNA和RNA处理酶及其底物之间的复合物进行统计分析。

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