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A Study on the Binding Ability of Truncated Aptamers for the Prostate Specific Antigen Using Both Computational and Experimental Approaches

机译:使用计算和实验方法研究前列腺特异性抗原截短适体的结合能力研究

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Prostate-specific antigen (PSA) test is a commonly used clinical examination to evaluate the risk of prostate cancer, with the antibodies used normally as the recognition molecules for measuring PSA levels in serum. Alternatively, aptamers that are able to bind target molecules with high affinity and specificity similar to antibodies could be generated much easier and cheaper than the production of antibodies. In this study, we used computaional and experimental approaches to select truncated PSA-binding aptamers generated from the sequence information of PSA-binding aptamers previously reported in a literature. Genetic algorithm, the analysis of secondary structure, and molecular simulation were utilized in the in silico analysis. The top 4 ranked sequecnes in silico analysis were evaluated through their PSA-binding ability on the quartz crystal microbalance (QCM) biosensor. Finally, We identified a truncated aptamer obtained from the selection showing a nearly 3.5-fold higher measured signal than the response produced by the best known DNA sequence in the QCM measurement.
机译:特异性前列腺特异性抗原(PSA)测试是一种常用的临床检查,以评估前列腺癌的风险,通常使用抗体作为用于测量血清中PSA水平的识别分子。或者,能够与抗体相似的具有高亲和力和特异性的靶分子的适体可以产生比抗体的产生更容易和便宜。在这项研究中,我们使用了从先前报道的PSA结合适体的序列信息中选择截短的PSA结合适体选择的截断的PSA结合体。遗传算法,二次结构分析和分子模拟中的硅分析。通过其PSA结合能力在石英晶体微稳定(QCM)生物传感器上的PSA结合能力评估二氧化硅分析中的排名第4类。最后,我们鉴定了从选择获得的截短的适体,示出了比QCM测量中最可知的DNA序列产生的响应更高的测量信号。

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