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Classification of DNA nucleotides with transverse tunneling currents

机译:具有横向隧穿电流的DNa核苷酸的分类

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摘要

It has been theoretically suggested and experimentally demonstrated that fast and low-cost sequencing of DNA, RNA, and peptide molecules might be achieved by passing such molecules between electrodes embedded in a nanochannel. The experimental realization of this scheme faces major challenges, however. In realistic liquid environments, typical currents in tunneling devices are of the order of picoamps. This corresponds to only six electrons per microsecond, and this number affects the integration time required to do current measurements in real experiments. This limits the speed of sequencing, though current fluctuations due to Brownian motion of the molecule average out during the required integration time. Moreover, data acquisition equipment introduces noise, and electronic filters create correlations in time-series data. We discuss how these effects must be included in the analysis of, e.g., the assignment of specific nucleobases to current signals. As the signals from different molecules overlap, unambiguous classification is impossible with a single measurement. We argue that the assignment of molecules to a signal is a standard pattern classification problem and calculation of the error rates is straightforward. The ideas presented here can be extended to other sequencing approaches of current interest.
机译:从理论上已经提出并通过实验证明,通过在纳米通道中嵌入的电极之间传递这样的分子,可以实现DNA,RNA和肽分子的快速低成本测序。然而,该方案的实验实现面临重大挑战。在现实的液体环境中,隧穿设备中的典型电流约为皮安。这相当于每微秒只有六个电子,这个数字会影响实际实验中进行电流测量所需的积分时间。这限制了测序的速度,尽管由于分子的布朗运动引起的电流波动在所需的积分时间内平均了下来。此外,数据采集设备会引入噪声,而电子滤波器会在时序数据中创建相关性。我们讨论了如何将这些效应包括在例如将特定核碱基分配给当前信号的分析中。由于来自不同分子的信号重叠,因此单次测量不可能进行明确的分类。我们认为将分子分配给信号是一个标准的模式分类问题,错误率的计算很简单。此处介绍的思想可以扩展到当前感兴趣的其他测序方法。

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