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PhD7Faster 2.0: predicting clones propagating faster from the Ph.D.-7 phage display library by coupling PseAAC and tripeptide composition

机译:PhD7Faster 2.0:通过偶联PseAAC和三肽组成预测从Ph.D.-7噬菌体展示文库更快繁殖的克隆

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摘要

Selection from phage display libraries empowers isolation of high-affinity ligands for various targets. However, this method also identifies propagation-related target-unrelated peptides (PrTUPs). These false positive hits appear because of their amplification advantages. In this report, we present PhD7Faster 2.0 for predicting fast-propagating clones from the Ph.D.-7 phage display library, which was developed based on the support vector machine. Feature selection was performed against PseAAC and tripeptide composition using the incremental feature selection method. Ten-fold cross-validation results show that PhD7Faster 2.0 succeeds a decent performance with the accuracy of 81.84%, the Matthews correlation coefficient of 0.64 and the area under the ROC curve of 0.90. The permutation test with 1,000 shuffles resulted in p < 0.001. We implemented PhD7Faster 2.0 into a publicly accessible web tool () and constructed standalone graphical user interface and command-line versions for different systems. The standalone PhD7Faster 2.0 is able to detect PrTUPs within small datasets as well as large-scale datasets. This makes PhD7Faster 2.0 an enhanced and powerful tool for scanning and reporting faster-growing clones from the Ph.D.-7 phage display library.
机译:从噬菌体展示库中进行选择可分离出各种目标的高亲和力配体。但是,此方法还可以识别与繁殖有关的靶标无关肽(PrTUPs)。这些假阳性结果的出现是由于其放大的优势。在此报告中,我们介绍了PhD7Faster 2.0,用于从Ph.D.-7噬菌体展示库预测快速繁殖的克隆,该库是基于支持向量机开发的。使用增量特征选择方法针对PseAAC和三肽组成进行特征选择。十倍交叉验证的结果表明,PhD7Faster 2.0具有不错的性能,准确度为81.84%,马修斯相关系数为0.64,ROC曲线下面积为0.90。 1,000次混洗的置换测试得出p <0.001。我们将PhD7Faster 2.0实施为可公开访问的Web工具(),并为不同系统构建了独立的图形用户界面和命令行版本。独立的PhD7Faster 2.0能够检测小型数据集和大型数据集内的PrTUP。这使PhD7Faster 2.0成为增强且功能强大的工具,可用于扫描和报告Ph.D.-7噬菌体展示库中增长较快的克隆。

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