ratio: Result of method getRatio on the complete dataset
In ChIPSeqSpike: ChIP-Seq data scaling according to spike-in control
Description
Usage
Format
Details
References
Description
Result of method getRatio on the complete dataset.
Usage
1
Format
matrix
Details
## Complete Dataset
The data used in this documentation represent a gold-standard example of the
importance of using spike-in controls with ChIP-Seq experiments. It uses
Drosophila Melanogaster chromatin as exogenous spike-in control to correct
experimental biases. Without spike-in control and using only RPM normalization,
proper differences of H3K79me2 histone modification in human Jurkat cells upon
EPZ5676 inhibitor treatment are not observed [1].
This dataset is made of bigwig and bam files of H3K79me2 ChIP-Seq data and
corresponding input DNA controls.
Bam files contain data aligned to the Human reference genome Hg19 or to the
Drosophila reference genome dm3. The latest is used to compute external
spike-in scaling factors. All above mentioned data are available at 0, 50 and
100 percent EPZ5676 inhibitor treatment (see vignette for data references).
References
[1] Orlando et al, "Quantitative ChIP-Seq normalization reveals global
modulation of the epigenome", Cell Rep, 2014.
ChIPSeqSpike documentation built on Nov. 8, 2020, 5:29 p.m.
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Description Usage Format Details References
Description
Result of method getRatio on the complete dataset.
Usage
1 |
Format
matrix
Details
## Complete Dataset
The data used in this documentation represent a gold-standard example of the importance of using spike-in controls with ChIP-Seq experiments. It uses Drosophila Melanogaster chromatin as exogenous spike-in control to correct experimental biases. Without spike-in control and using only RPM normalization, proper differences of H3K79me2 histone modification in human Jurkat cells upon EPZ5676 inhibitor treatment are not observed [1].
This dataset is made of bigwig and bam files of H3K79me2 ChIP-Seq data and corresponding input DNA controls. Bam files contain data aligned to the Human reference genome Hg19 or to the Drosophila reference genome dm3. The latest is used to compute external spike-in scaling factors. All above mentioned data are available at 0, 50 and 100 percent EPZ5676 inhibitor treatment (see vignette for data references).
References
[1] Orlando et al, "Quantitative ChIP-Seq normalization reveals global modulation of the epigenome", Cell Rep, 2014.
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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