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Short oligonucleotide probes containing G-stacks display abnormal binding affinity on Affymetrix microarrays

机译:包含G-stacks的短寡核苷酸探针在Affymetrix微阵列上显示出异常的结合亲和力

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Motivation: In microarray experiments, probe design is critical to the specific and accurate measurement of target concentrations. Current designs select suitable probes through in silico scanning of transcriptome/genome based on first principles. However, due to lack of tools, the observed microarray data have not been used to assess the performance of individual probes to provide feedback to improve future designs. Results: In this study, we describe a probe performance assessment method based on the concordance of the observed signals from probes that share common targets. Using this method, we found that probes containing multiple guanines in a row (G-stacks) have abnormal binding behavior compared with other probes, both in gene expression assays and genotyping assays using Affymetrix microarrays. These probes are less likely to covary with other probes that interrogate the same genes. Moreover, we found that these probes are much more likely to produce outliers when fitting the observed signals according to the positional dependent nearest neighbor model, which gives reasonable estimates of binding affinity for most other probes. These results suggest that probes containing G-stacks tend to have increased cross hybridization signals and reduced target-specific hybridization signals, presumably due to multiplex binding forming G-quartet structures. Our findings are expected to be useful in microarray design and data analysis.
机译:动机:在微阵列实验中,探针设计对于目标浓度的特异性和精确测量至关重要。当前的设计基于第一原理通过对转录组/基因组进行计算机扫描来选择合适的探针。然而,由于缺乏工具,所观察到的微阵列数据尚未用于评估单个探针的性能以提供反馈以改进未来的设计。结果:在这项研究中,我们基于共享目标的探针的观察信号的一致性描述了一种探针性能评估方法。使用这种方法,我们发现在基因表达分析和使用Affymetrix微阵列进行基因分型分析中,连续包含多个鸟嘌呤的探针(G堆栈)与其他探针相比具有异常的结合行为。这些探针不太可能与询问相同基因的其他探针共存。此外,我们发现,根据位置相关的最近邻居模型拟合观察到的信号时,这些探针更有可能产生离群值,这可以合理估计大多数其他探针的结合亲和力。这些结果表明,包含G-堆栈的探针倾向于具有增加的交叉杂交信号和减少的靶标特异性杂交信号,这可能是由于形成G-四重结构的多重结合所致。我们的发现有望用于微阵列设计和数据分析。

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