data4: Input data (matrix) for condition B
In ChIPtest: Nonparametric Methods for Identifying Differential Enrichment Regions with ChIP-Seq Data
Description
Usage
Format
Source
References
Examples
Description
In order to identify the genes that show differential histone modification levels between the two conditions, condition A and condition B, ChIPtest consider the upstream 5000 bp region and downstream 2000 bp region around the transcription start site (TSS) for each gene and divide the regions into 280 bins of 25 bps. Since the two ChIP-seq samples are usually sequenced at different depths (total number of reads), the counts were rescaled according to the sequencing depth ratio. In this example, suppose that there are 5 genes and for each gene, there are 280 observations. The input data matrix has 5 rows and 280 columns. Each row represents for one gene, and each column represents for number of short reads covered at one bin after rescaling.
Usage
1
Format
The format is:
num [1:5, 1:280] 0 0 0 0 0 0 0 0 0 0 ...
- attr(*, "dimnames")=List of 2
..$ : chr [1:5] "1" "2" "3" "4" ...
..$ : chr [1:280] "V3" "V4" "V5" "V6" ...
Source
T.S. Mikkelsen, et al. Comparative Epigenomic Analysis of Murine and Human Adipogenesis. Cell, 143 (156-169): 1156-1166 (2010)
References
Qian Wu, Kyoung-Jae Won and Hongzhe Li. (2015) Nonparametric Methods for Identifying Differential Enrichment Regions with ChIP-seq Data. Cancer Informatics,14 (Suppl 1), 11-22
Examples
1
ChIPtest documentation built on May 2, 2019, 3:37 p.m.
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Description Usage Format Source References Examples
Description
In order to identify the genes that show differential histone modification levels between the two conditions, condition A and condition B, ChIPtest consider the upstream 5000 bp region and downstream 2000 bp region around the transcription start site (TSS) for each gene and divide the regions into 280 bins of 25 bps. Since the two ChIP-seq samples are usually sequenced at different depths (total number of reads), the counts were rescaled according to the sequencing depth ratio. In this example, suppose that there are 5 genes and for each gene, there are 280 observations. The input data matrix has 5 rows and 280 columns. Each row represents for one gene, and each column represents for number of short reads covered at one bin after rescaling.
Usage
1 |
Format
The format is: num [1:5, 1:280] 0 0 0 0 0 0 0 0 0 0 ... - attr(*, "dimnames")=List of 2 ..$ : chr [1:5] "1" "2" "3" "4" ... ..$ : chr [1:280] "V3" "V4" "V5" "V6" ...
Source
T.S. Mikkelsen, et al. Comparative Epigenomic Analysis of Murine and Human Adipogenesis. Cell, 143 (156-169): 1156-1166 (2010)
References
Qian Wu, Kyoung-Jae Won and Hongzhe Li. (2015) Nonparametric Methods for Identifying Differential Enrichment Regions with ChIP-seq Data. Cancer Informatics,14 (Suppl 1), 11-22
Examples
1 |
R Package Documentation
Browse R Packages
We want your feedback!
Note that we can't provide technical support on individual packages. You should contact the package authors for that.
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