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a normalization strategy for comparing tag count data比较标签计数数据的标准化战略
Kadota et al. Algorithms for Molecular Biology 2012, 7:5
/content/7/1/5
RESEARCH Open Access
A normalization strategy for comparing tag count
data
Koji Kadota1,2*, Tomoaki Nishiyama3 and Kentaro Shimizu1
Abstract
Background: High-throughput sequencing, such as ribonucleic acid sequencing (RNA-seq) and chromatin
immunoprecipitation sequencing (ChIP-seq) analyses, enables various features of organisms to be compared
through tag counts. Recent studies have demonstrated that the normalization step for RNA-seq data is critical for a
more accurate subsequent analysis of differential gene expression. Development of a more robust normalization
method is desirable for identifying the true difference in tag count data.
Results: We describe a strategy for normalizing tag count data, focusing on RNA-seq. The key concept is to
remove data assigned as potential differentially expressed genes (DEGs) before calculating the normalization factor.
Several R packages for identifying DEGs are currently available, and each package uses its own normalization
method and gene ranking algorithm. We compared a total of eight package combinations: four R packages (edgeR,
DESeq, baySeq, and NBPSeq) with their default normalization settings and with our normalization strategy. Many
synthetic datasets under various scenarios were evaluated on the basis of the area under the curve (AUC) as a
measure for both sensitivity and specificity. We found that packages using our strategy in the data normalization
step overall performed well. This result was also observed for a real experimental dataset.
Conclusion: Our results showed that the elimination of potential DEGs is essential for more accurate normalization
of RNA-seq data. The concept of this normalization strategy can widely be applied to other types of tag count
data and to micro
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