MAnorm2 is designed for normalizing and comparing ChIP-seq
signals across individual samples or groups of samples. The latest
version of MAnorm2 is always available in the CRAN repository and can thus be
easily installed by typing install.packages("MAnorm2")
in
an R session.
For older versions of MAnorm2, select a package from under the
dist
folder, download it, and type
install.packages("/path/to/the/package", repos = NULL)
. In
this way, you may need to pre-install some dependencies of MAnorm2. The
current dependencies of the latest MAnorm2 version include locfit (>=
1.5.9), scales (>= 0.3.0), and statmod (>= 1.4.34). All these
packages are available in the CRAN repository. For dependencies
of other MAnorm2 versions, refer to the Imports
field in
the corresponding DESCRIPTION
file.
Sections below give a brief description of the application scope of MAnorm2 as well as its capability. For a full documentation of MAnorm2, download the HTML version of its vignette from here and use a browser to open it, or type the following code in an R session after installing MAnorm2:
browseVignettes("MAnorm2")
For employing the machinery implemented in MAnorm2, you need to prepare a table that profiles the ChIP-seq signal in each of a list of genomic intervals for each of a set of ChIP-seq samples. The following table provides such an instance:
chrom | start | end | s1.read_cnt | s2.read_cnt | s1.occupancy | s2.occupancy |
---|---|---|---|---|---|---|
chr1 | 28112 | 29788 | 115 | 4 | 1 | 0 |
chr1 | 164156 | 166417 | 233 | 194 | 1 | 1 |
chr1 | 166417 | 168417 | 465 | 577 | 1 | 1 |
chr1 | 168417 | 169906 | 15 | 34 | 0 | 1 |
(See the H3K27Ac
dataset bundled with MAnorm2 for
another example, and type library(MAnorm2); ?H3K27Ac
in an
R session for a detailed description of it.)
To be specific, each row of the table represents a genomic interval;
each of the read_cnt
variables corresponds to a ChIP-seq
sample and gives the numbers of reads from the sample that fall within
the genomic intervals (i.e., the raw read counts); the
occupancy
variables correspond to the read_cnt
variables one by one and specify the occupancy status of each genomic
interval in each sample. Note that an occupancy status of 1 indicates
the interval is enriched with reads in the sample (compared with, for
example, the surrounding genomic regions or the corresponding input
sample). In practice, the occupancy status of a genomic interval in a
certain ChIP-seq sample could be determined by its overlap with the peaks
of the sample. Note also that MAnorm2 refers to an interval as occupied
by a sample if the interval is enriched with reads in the sample.
MAnorm2_utils is specifically designed to coordinate with MAnorm2, and we strongly recommend using it to create input tables of MAnorm2.
Although MAnorm2 has been designed to process ChIP-seq data, it could be applied in principle to the analysis of any type of data with a similar structure, including DNase-seq, ATAC-seq and RNA-seq data. The only problem associated with such extensions is how to naturally define “peaks” for specific data types.
Most of the peak callers originally devised for ChIP-seq data (e.g., MACS 1.4) also work for DNase-seq and ATAC-seq data. For RNA-seq data, each row of the input table should stand for a gene, and we recommend setting a cutoff (e.g., 20) of raw read count to define “peak” genes.
In spite of the discrete nature of read counts, MAnorm2 uses continuous distribution to model ChIP-seq data by first transforming raw read counts into raw signal intensities. By default, MAnorm2 completes the transformation by simply adding an offset count to each raw count and taking a base-2 logarithm. Practical ChIP-seq data sets, however, may be associated with various confounding factors, including batch effects, local sequence compositions and background signals measured by input samples. On this account, functions in MAnorm2 have been designed to be independent of the specific transformation employed. And any methods for correcting for confounding factors could be applied before invoking MAnorm2, as long as the resulting signal intensities could be approximately modeled as following the normal distribution (in particular, consider carefully whether it is necessary to apply a logarithmic transformation in the final step).
The primary reason for which MAnorm2 models ChIP-seq signals as continuous random variables is that the mathematical theory of count distributions is far less tractable than that of the normal distribution. For example, current statistical methods based on the negative binomial distribution are frequently relied on approximations of various kinds. Specifically, variance (or dispersion) estimates for individual genomic intervals are typically treated as known parameters, and their uncertainty can hardly be incorporated into the statistical tests for identifying differential signals.
Besides, after an extensive correction for confounding factors, the resulting data range is almost certainly not limited to non-negative integers, and the data may have lost their discrete nature and be more akin to a continuous distribution. Moreover, transforming read counts towards the normal distribution unlocks the application of a large repository of mature statistical methods that are initially developed for analyzing continuous measurements (e.g., intensity data from microarray experiments). Refer to the voom article for a detailed discussion of this topic.
MAnorm2 implements a robust method for normalizing raw signal intensities across any number of ChIP-seq samples.
Technically, it considers the common peak regions of two ChIP-seq samples (i.e., the genomic intervals occupied by both samples; see also the section of Format of Input Data) to have globally invariant signals between them. Based on this assumption, MAnorm2 applies a linear transformation to the raw signal intensities of one of the two samples such that
This procedure is for normalizing a pair of ChIP-seq samples. It can be extended to normalization of any number of samples so that the normalized signal intensities are comparable across all of them. For more information regarding the normalization method implemented in MAnorm2, type the following code in an R session after installing it:
library(MAnorm2)
?normalize ?normBioCond
MAnorm2 designs a self-contained system of utility functions for
calling differential ChIP-seq signals between two or more biological
conditions, each with or without replicate samples. It also implements a
method named HyperChIP for calling hypervariable ChIP-seq signals across
samples. To be noted, the framework implemented in MAnorm2 for
differential and hypervariable analyses requires the input signal
intensities to have been normalized but is independent of the specific
normalization method. This means that any normalization and/or bias
correction tools could be adapted to MAnorm2, as long as the resulting
signal measurements are suited to be modeled by normal distribution. For
example, for highly regular samples, you might want to perform the
normalization based on their size factors (refer to the
normalizeBySizeFactors
function in MAnorm2 for
details).
Technically, MAnorm2 has implemented an S3 class named “bioCond” for grouping ChIP-seq samples belonging to the same biological condition, and it has devised a number of functions for handling objects of this class. Taking advantage of these functions, you can
Note that, for the samples grouped into a bioCond, MAnorm2 models the relationship between observed mean signal intensities at individual intervals and the associated (observed) variances. In practice, this modeling strategy could compensate for the lack of sufficient replicates for deriving accurate variance estimates for individual intervals. And each of the above analyses takes advantage of the modeling of mean-variance trend to improve variance estimation.
For an overview of the interface functions provided by MAnorm2, type the following code in an R session after installing it:
library(MAnorm2)
?MAnorm2
To cite the MAnorm2 package in publications, please use
Tu, S., et al., MAnorm2 for quantitatively comparing groups of ChIP-seq samples. Genome Res, 2021. 31(1): p. 131-145.
If you have performed MA normalization with a pseudo-reference profile as baseline, or have employed a Winsorization-based robust parameter estimation framework, or have performed a hypervariable analysis, please cite additionally
Chen, H., et al., HyperChIP: identification of hypervariable signals across ChIP-seq or ATAC-seq samples. Genome Biol, 2022. 23(1): p. 62.