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An improved readout method of molecular computation based on real-time PCR implemented on DNA Engine Opticon 2 System

机译:基于DNA Engine Opticon 2系统的基于实时PCR的分子计算的改进读出方法

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A readout approach for the Hamiltonian Path Problem (HPP) in DNA computing based on the real-time polymerase chain reaction (PCR) is re-implemented on DNA Engine Opticon 2 System. Several types of fluorescent probes and detection mechanisms are currently employed in real-time PCR, including SYBR Green, molecular beacons, and hybridization probes. Based on the new approach, real-time amplification performed using the TagMan probes is adopted, as the TagMan detection mechanism can be exploited for the design and development of the proposed readout approach. In this study, double-stranded DNA molecules of length 140 base-pairs are selected as the input molecules, which represent the solving path for an HPP instance. These input molecules are prepared via the self-assembly of 20-mer and 30-mer single-stranded DNAs, by parallel overlap assembly. The proposed readout approach consists of two steps: real-time amplification in vitro using TagMan-based real-time PCR, followed by information processing in silico to assess the results of real-time amplification, which in turn, enables extraction of the Hamiltonian path. The experimental result is compared with that of previously implementation on Roche LightCycler System. Experimental results establish an easier method to interpret the output of real-time PCR for the subsequent in silico information processing.
机译:在DNA Engine Opticon 2系统上重新实现了基于实时聚合酶链反应(PCR)的DNA计算中哈密顿路径问题(HPP)的读出方法。当前,实时PCR中采用了几种类型的荧光探针和检测机制,包括SYBR Green,分子信标和杂交探针。基于新方法,采用了使用TagMan探针执行的实时扩增,因为可以利用TagMan检测机制来设计和开发所建议的读出方法。在这项研究中,选择长度为140个碱基对的双链DNA分子作为输入分子,代表了HPP实例的求解路径。这些输入分子是通过20-mer和30-mer单链DNA的自组装,通过平行重叠组装而制备的。拟议的读出方法包括两个步骤:使用基于TagMan的实时PCR在体外进行实时扩增,然后进行计算机信息处理以评估实时扩增的结果,从而可以提取汉密尔顿路径。将实验结果与先前在Roche LightCycler System上实施的结果进行了比较。实验结果建立了一种更容易的方法,可为后续的计算机信息处理解释实时PCR的输出。

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