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Temperature and electrolyte optimization of the α-hemolysin latch sensing zone for detection of base modification in double-stranded DNA

机译:用于检测双链DNA碱基修饰的α-溶血素闩锁传感区的温度和电解质优化

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摘要

The latch region of the wild-type protein pore α-hemolysin (α-HL) constitutes a sensing zone for individual abasic sites (and furan analogs) in double-stranded DNA (dsDNA). The presence of an abasic site or furan within a DNA duplex, electrophoretically captured in the α-HL vestibule and positioned at the latch region, can be detected based on the current blockage prior to duplex unzipping. We investigated variations in blockage current as a function of temperature (12–35°C) and KCl concentration (0.15–1.0 M) to understand the origin of the current signature and to optimize conditions for identifying the base modification. In 1 M KCl solution, substitution of a furan for a cytosine base in the latch region results in an ∼8 kJ mol−1 decrease in the activation energy for ion transport through the protein pore. This corresponds to a readily measured ∼2 pA increase in current at room temperature. Optimal resolution for detecting the presence of a furan in the latch region is achieved at lower KCl concentrations, where the noise in the measured blockage current is significantly lower. The noise associated with the blockage current also depends on the stability of the duplex (as measured from the melting temperature), where a greater noise in the measured blockage current is observed for less stable duplexes.
机译:野生型蛋白孔α-溶血素(α-HL)的闩锁区域构成了双链DNA(dsDNA)中单个无碱基位点(和呋喃类似物)的感应区。可以根据双链体解链前的电流阻滞,检测DNA双链体中无碱基位点或呋喃的存在,该片段通过电泳捕获在α-HL前庭中并位于闩锁区域。我们研究了阻塞电流随温度(12–35°C)和KCl浓度(0.15–1.0 M)的变化,以了解电流信号的起源并优化用于鉴定碱基修饰的条件。在1 M KCl溶液中,用呋喃取代闩锁区域中的胞嘧啶碱基会导致离子通过蛋白质孔传输的活化能降低约8 kJ mol-1。这相当于在室温下容易测得的电流增加约2 pA。在较低的KCl浓度下,可以实现用于检测闩锁区域中呋喃的最佳分辨率,在这种情况下,测得的阻断电流中的噪声明显较低。与阻塞电流相关的噪声还取决于双工的稳定性(从熔化温度测量),对于较不稳定的双工,在测量的阻塞电流中观察到较大的噪声。

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