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比较分析 mRNA 特征对局部核糖体分析读密度相对影响的研究

Comparative survey of the relative impact of mRNA features on local ribosome profiling read density.

机构信息

School of Biochemistry and Cell Biology, University College Cork, Cork, Ireland.

Belozersky Institute of Physico-Chemical Biology, Lomonosov Moscow State University, Moscow 119234, Russia.

出版信息

Nat Commun. 2016 Oct 4;7:12915. doi: 10.1038/ncomms12915.

Abstract

Ribosome profiling (Ribo-seq), a promising technology for exploring ribosome decoding rates, is characterized by the presence of infrequent high peaks in ribosome footprint density and by long alignment gaps. Here, to reduce the impact of data heterogeneity we introduce a simple normalization method, Ribo-seq Unit Step Transformation (RUST). RUST is robust and outperforms other normalization techniques in the presence of heterogeneous noise. We illustrate how RUST can be used for identifying mRNA sequence features that affect ribosome footprint densities globally. We show that a few parameters extracted with RUST are sufficient for predicting experimental densities with high accuracy. Importantly the application of RUST to 30 publicly available Ribo-seq data sets revealed a substantial variation in sequence determinants of ribosome footprint frequencies, questioning the reliability of Ribo-seq as an accurate representation of local ribosome densities without prior quality control. This emphasizes our incomplete understanding of how protocol parameters affect ribosome footprint densities.

摘要

核糖体图谱(Ribo-seq)是一种很有前途的技术,可用于探索核糖体解码速率,其特征是核糖体足迹密度中存在罕见的高峰值和长的比对间隙。在这里,为了降低数据异质性的影响,我们引入了一种简单的归一化方法,核糖体图谱单位阶跃变换(RUST)。RUST 稳健性好,在存在异质噪声的情况下优于其他归一化技术。我们说明了如何使用 RUST 来识别影响全局核糖体足迹密度的 mRNA 序列特征。我们表明,使用 RUST 提取的几个参数足以高精度地预测实验密度。重要的是,RUST 应用于 30 个公开的 Ribo-seq 数据集,揭示了核糖体足迹频率的序列决定因素存在很大差异,这使得人们对 Ribo-seq 作为局部核糖体密度的准确表示而无需事先进行质量控制的可靠性产生了质疑。这强调了我们对协议参数如何影响核糖体足迹密度的理解还不完整。

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