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A Peak Alignment Algorithm with Novel Improvements In Application to Electropherogram Analysis

机译:一种新改进的峰对准算法在电泳图分析中的应用

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摘要

Alignment of peaks in electropherograms or chromatograms obtained from experimental techniques such capillary electrophoresis remains a significant challenge. Accurate alignment is critical for accurate interpretation of various classes of nucleic acid analysis technologies, including conventional DNA sequencing and new RNA structure probing technologies. We have developed an automated alignment algorithm based on dynamic programming to align multiple-peak time-series data both globally and locally. This algorithm relies on a new peak similarity measure and other features such as time penalties, global constraints, and minimum-similarity scores and results in rapid, highly accurate comparisons of complex time-series datasets. As a demonstrative case study, the developed algorithm was applied to analysis of capillary electrophoresis data from a Selective 2′-Hydroxyl Acylation analyzed by Primer Extension (SHAPE) evaluation of RNA secondary structure. The algorithm yielded robust analysis of challenging SHAPE probing data. Experimental results show that the peak alignment algorithm corrects retention time variation efficiently due to the presence of fluorescent tags on fragments and differences in capillaries. The tools can be readily adapted for the analysis other biological datasets in which peak retention times vary.
机译:从实验技术(例如毛细管电泳)获得的电泳图或色谱图中的峰对齐仍然是一个重大挑战。准确的比对对于准确解释各种类型的核酸分析技术至关重要,包括常规的DNA测序和新的RNA结构探测技术。我们已经开发了一种基于动态编程的自动对齐算法,可以在全球和本地对齐多峰时间序列数据。该算法依赖于新的峰值相似性度量和其他功能,例如时间惩罚,全局约束和最小相似性得分,并且可以对复杂的时间序列数据集进行快速,高度准确的比较。作为演示案例研究,将开发的算法应用于通过选择性引物扩展(SHAPE)评估RNA二级结构分析的选择性2'-羟酰酰化反应中的毛细管电泳数据。该算法对具有挑战性的SHAPE探测数据进行了稳健的分析。实验结果表明,由于碎片上存在荧光标签以及毛细管中的差异,峰对齐算法可以有效地校正保留时间变化。这些工具可以轻松地用于分析峰保留时间变化的其他生物学数据集。

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