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Nucleosome Dynamics CLI

This repository includes the set of R programs implementing 'Nucleosome Dynamics' analyses.


Landing page http://mmb.irbbarcelona.org/NucleosomeDynamics

Table of contents


Nucleosome Dynamics

Nucleosome positioning plays a major role in transcriptional regulation DNA replication and DNA repair. The Nucleosome Dynamics CLI offers different R scripts to analyze nucleosome positioning from MNase-seq experimental data and to compare experiments to account for the transient and dynamic nature of nucleosomes under different cellular states.

The main analyses are performed with nucleR and NucDyn R packages:

  • nucleR performs Fourier transform filtering and peak calling to efficiently and accurately find the location of nucleosomes and classify them according to their fuzziness.
  • NucDyn detects changes in nucleosome architectures between two MNase-seq experiments. It identifies nucleosomes’ insertions, evictions and shifts at the read level.

'Nucleosome Dynamics' also offers other nucleosome-related analyses:

  • NFR: location of nucleosome-free regions
  • TSS: classification of transcription start sites based on the surrounding nucleosomes
  • Periodicity: study of nucleosome phasing at gene level
  • Stiffness: computation of stiffness of the nucleosomes derived from fitting a Gaussian function to nucleosome profiles

Additionally, after computing all the analyses, a series of statistics (plots and tables) can be computed to obtain:

  • genome-wide values for all calculations
  • counts and averages at the gene level

'Nucleosome Dynamics CLI' is not only offered throught the native R interface, but a number of other implementation have been prepared in order to reach also non-R users. These implementations include two web-based platforms (MuGVRE and Galaxy) and two containerized installations (docker and singularity)

    ┌──────────────────────────────────────────────────────────┐
    │                   Nucleomose Dynamics                    │
    │                                                          │
    │       ┌───────────────┐         ┌───────────────┐        │
    │       │    nucleR     │         │     NucDyn    │        │
    │       └───────|───────┘         └────────|──────┘        │
    │               │                          │               │
    │           ┌─────────────────────────────────┐            │
    │           │    Nucleosome Dynamics CLI      │            │
    |           └┌──────────────────────┐────────┐┘            │
    │            │                      │        │             │
    │┌───────────└┐ ┌───────────┐ ┌─────└─────┐ ┌└────────────┐│
    ││   MuGVRE   │ │   Galaxy  │-│   Docker  │ │ Singularity ││
    │└────────────┘ └───────────┘ └───────────┘ └─────────────┘│
    └──────────────────────────────────────────────────────────┘

Requirements

  • R >= 3.5
  • R packages
    • NucDyn
    • nucleR
  • UCSC wig utilities
    • wigToBigWig
    • bigWigToWig
    • fetchChromSizes

Installation

The instructions on how to install 'Nucleosome Dynamics CLI' are detailed at here.

Input data

The primary data for 'Nucleosome Dynamics CLI' are MNase-seq aligned and sorted reads in BAM format. Additionally, as detailed in the Usage section below, some data for the reference genome are also required. Go to test/data for a detailed description on such data. The folder also contains an example data set for ilustrating the R program usage.

Running Nucleosome Dynamics CLI

Simply run each of the analysis as follows:

Rscript bin/[analysis].R [analysis_arguments]

Where analysis.R are:

[analysis] Description
readBAM Read Aligned MSase-seq BAM into a RData structure (required for further processing)
nucleR Determine the positions of the nucleosomes across the genome
nucDyn Compare of two MNase-seq experiments to detect nucleosome architecture local changes
NFR Detect short regions depleted of nucleosomes
txstart Classify TSS according to the properties of nucleosomes +1 and -1
periodicity Compute periodic properties of nucleosomes inside gene bodies
stiffness Estimate an aparent stiffness for each nucleosome obtained by fitting a Gaussian distribution to the nucleosome coverage


Additionally, each analysis has a statistics module that creates a report (tabular or graphical) for summarising the calculation. After running each analysis, obtain the corresponding summary statistics as follows:

Rscript statistics/[analysis_stats].R [analysis_stats_arguments]

Available analysis_stats.R are:

[analysis_stats] Description
nucleR Nucleosome call fuzziness statistics
NFR Nucleosome Free Regions statistics
txstart TSS classification statistics
periodicity Statistics on nucleosome periodicity along gene bodies
stiffness Statistics on stiffness values
nucDyn Statistics on nucleosome changes detected by NucDyn

The Usage section below describes the arguments for each individual analysis and, similarly, the Results section includes a description of the sequence annotations files (GFF or bigWig) generated.

Example

Nucleosome calls can be obtained with 'nucleR' from a BAM file of paired MNase-seq sequencing fragments. The MNase-seq reads in BAM format first have to be converted to RData format using readBAM:

Rscript bin/readBAM.R --input test/data/cellcycleG2_chrII.bam --output test/data/cellcycleG2_chrII.RData --type paired

Once the RData is generated, nucleosome calling with nucleR can be performed as follows:

Rscript bin/nucleR.R --input test/data/cellcycleG2_chrII.RData --output test/data/NR_cellcycleG2_chrII.gff --type paired 

For obtaining a statistical report of the 'nucleR', the resulting GFF file is passed as an argument into statistics/nucleR.R:

Rscript statistics/nucleR.R --input test/data/NR_cellcycleG2_chrII.gff --genome test/data/refGenomes/R64-1-1/genes.gff --out_genes test/data/NR_cellcycleG2_chrII_genes.csv --out_gw test/data/N/NR_cellcycleG2_chrII_stat.csv

Check the argument descriptions for each particular analysis at the Usage section. The 'nucleR' execution will generate the NR_cellcycleG2_chrII.gff track file with the detected nucleosome positions and a number of scores described in the Results section. Most of the sequence browsers can visualize it, for instance, JBrowse.

Usage

Analyses usage

bin/readBAM.R

Rscript bin/readBAM.R --input {bam} --output {RData} --type (single|paired)
    --input
            Mapped sequences file in BAM format
    --output
            RData file
    --type
            Type of sequence data: single|paired

bin/nucleR

Rscript bin/**nucleR.R** --input {RData} --output {gff} --type (single|PAIRED)  \
[--minoverlap {int} --width {int} --dyad_length {int} --hthresh {double} --wthresh {double} --pcKeepComp {double} --fdrOverAmp {double} --components {int} --fragmentLen {int} --trim {int} --threshold {logical} --thresholdValue {int} --thresholdPercentage {double} --chr STR --start {int} --end {int} ]
    --input: 
            Input BAM file (RData format)
    --output:
            Nucleosome calls in GFF format. Annotations: Score_weight (0-1), Score_height (0-1), class (W, F, uncertain)
    --type
            Type of sequence data: single|paired
    --minoverlap: 
            Minimum number of overlapping base pairs in two nucleosome calls for them to be merged into one (bp). Optional, default 80.
    --width: 
            Width given to nucleosome calls previous to merging (bp). Optional. Default 147.
    --dyad_length: 
            Number of bases around the dyad of the nucleosome calls to be used for nucleosome scoring (bp). Optional, default 50.
    --hthresh: 
            Height threshold (between 0 and 1) to classify (in combination with width threshold) a nucleosome as either fuzzy or well-positioned according to the number of reads in the dyad of the nucleosome call. Nucleosomes below this value (that is, nucleosomes with low coverage) will be defined as fuzzy. Optional, default 0.4.
    --wthresh: 
            Width threshold (between 0 and 1) to classify (in combination with height threshold) a nucleosome as either fuzzy or well-positioned according to the disperion of the reads around the dyad. Nucleosomes below this value (that is, nucleosome calls not sharp enough) will be defined as fuzzy. Optional, default 0.6
    --pcKeepComp
            Parameter used in the coverage smoothing when Fourier transformation is applied. Number of components to select with respect to the total size of the sample. Allowed values are numeric (in range 0:1) for manual setting, or 'auto' for automatic detection. Optional, default 0.02.
    --fdrOverAmp
            Threshold to filter over-amplified reads, as defined in filterDuplReads function of htSetqTools R package. Optional, default 0.05. 
    --components
            Number of negative binomials that will be used to filter duplicated reads, as defined in filterDuplReads function of htSetqTools R package. Optional, default 1.
    --fragmentLen
            Maximum fragment length allowed (bp). Optional, default 170.
    --trim
            Number of bases around the center of each fragment (bp) to use for peak calling. Optional, default 50.
    --threshold
            Defines what threshold should be used to filter out non-significant nucleosome calls. If set to TRUE, the percentage value is considered (--thresholdPercentage). If set to FALSE, the absolute value (--thresholdValue) is used. Optional, default TRUE.
    --thresholdValue
            Absolute value to filter out nucleosome calls. It is the minimum number of reads (coverage) in a nucleosome call expressed as reads per million of mapped reads. Optional, default 10.
    --thresholdPercentage: 
            Percentile of coverage in the experiment used as threshold to filter out nucleosome calls (i.e., '25%' would mean that only peaks with coverage in the 1st quantile would be considered). Optional, default 35(%)
    --chr
            Chromosome to consider for the analysis in the given input file. By default, all the genomic range is considered. Optional, default NULL. 
    --start
            Start genomic position to consider for the analysis in the given input file. By default, all the genomic range is considered. Optional, default NULL. 
    --end
            End genomic position to consider for the analysis in the given input file. By default, all the genomic range is considered. Optional, default NULL. 

bin/nucDyn.R

Rscript bin/nucDyn.R  --input1 {RData} --input2 {RData} --calls1 {gff} --calls2 {gff} --outputGff {gff} --outputBigWig {bw}  --genome {chrom.sizes} \
[ --range {str} --plotRData {RData} --maxDiff {int} --maxLen {int} --shift_min_nreads {int} --shift_threshold {double} --indel_min_nreads {int} --indel_threshold {double} --cores {int} --equal_size (logical) --readSize {int} ]
    --input1, --input2
            Input BAM from MNase-seq in RData format (from readBAM)
    --calls1, --calls2
            Nucleosome calls in GFF format as obtained from nucleR
    -outputGff
            Output of NucDyn in GFF format: position of evictions, inclusions, shifts.
    --outputBigWig {bw}
            Output of NucDyn in BigWig format: -log10 of the p-value of the significance of the differences found.
    --genome {chrom.sizes}
            Chromosome sizes from reference genome
    --range (All|chr|chr:start-end)
            Genomic range to be analyzed. All: all genome; chr: a whole chromosome; chr:start-end: a specific region given the coordinates. Optional, default All.
    --plotRData {RData}
            Save all the detected changes at the fragment level in RData format for posterior plotting. Optional, default NULL (no RData is saved).
    --maxDiff
            Maximum distance between the centers of two fragments for them to be paired as shifts. (bp) Optional, default 70.
    --maxLen
            This value is used in a preliminar filtering. Fragments longer than this will be filtered out, since they are likely the result of MNase under-digestion and represent two or more nucleosomes (bp). Optional, default 140.
    --shift_min_nreads
            Minimum number of shifted reads for a shift hostspot to be reported {int}. Optional, default 3.
    --shift_threshold
            Threshold applied to the shift hostpots. Only hotspots with a score better than the value will be reported. Notice the score has to be lower than the threshold, since these numbers represent p-values {float}. Optional, default 0.1.
    --indel_min_nreads
            Minimum number of removed/included reads for an insertion or eviction hostspot to be reported {int}. Optional, default 3.
    --indel_threshold
            Threshold applied to the inclusion and eviction hostpots. Only hotspots with a score better than the value will be reported. Notice the score has to be lower than the threshold, since these numbers represent p-values {float}. Optional, default 0.05.
    --cores 
            Number of computer threads. Optional, default 1.
    --equal_size
            Trim all fragments to the same size. Optional, default FALSE.
    --readSize  
            Length to which all reads will be set in case `equalSize` is `TRUE`. It is ignored when `equalSize` is set to `FALSE`. Optional, default 140.

bin/NFR.R

Rscript bin/NFR.R  --input {gff} --output {gff} [--minwidth {int} --threshold {int}  ]
    --input 
            Nucleosome calls in GFF format as obtained from nucleR.
    --output {gff} 
            Nucleosome Free Regions in GFF format.
    --minwidth 
            Minimum length (bp). Optional, default 110bp.
    --threshold 
            Maximum length (bp). Optional, default 400bp.

bin/txstart.R

Rscript bin/txstart.R  --calls {gff} --genome {gff} --output {gff} \
[ --window {int} --open_thresh {int} --cores {int} --p1.max.downstream {int} ]
    --calls
            Nucleosome calls as obtained form nucleR. GFF format
    --genome
            Gene positions in the reference genome. GFF Format
    --output
            Classification of TSS according to nucleosome -1 and +1. GFF format.
    --window 
            Number of nucleotides on each side of the TSS where -1 and +1 nucleosomes are searched for. Optional, default 300.
    --open_thresh
            Distance between nucleosomes -1 and +1 to discriminate between 'open' and 'close' classes. Optional, default 215.
    --cores
            Number of computer threads. Optional, default 1.
    --p1.max.downstream
            Maximum distance upstream from the TSS to look for +1 nucleosome. Optional, default 20.

bin/periodicity.R

Rscript bin/periodicity.R --calls {gff} --reads {RData} --type (single|paired) --gffOutput {gff} --bwOutput {bw} --genes {gff} --chrom_sizes {chrom.sizes} \
[--periodicity {int} --cores {int} ]
    --calls
            Nucleosome calls in GFF format as obtained from nucleR.
    --reads
            Sequence Reads in RData format as obtained from readBAM.
    --type 
            Type of reads (single|paired)
    --gffOutput
            Periodicity output in GFF format.
    --bwOutput
            Periodicity output in BigWig format.
    --genes
            Position of genes in reference genome. GFF format
    --chrom_sizes
            Chromosome sizes file in the reference genome.
    --periodicity
            Average distance between two consecutive nucleosomes. It is used as the period of the nucleosome coverage signal. It should be defined according to the nucleosome repeat length in the corresponding cell type. Optional, default 165.
    --cores
            Number of computer threads. Optional, default 1.

bin/stiffness.R

Rscript bin/stiffness.R --calls {gff} --reads {RData} --output {gff} \
[ --range {str} --t {double}] ]
    --calls
            Nucleosome calls in GFF format as obtained from nucleR.
    --reads
            Sequence data in RData format as obtained from readBAM.
    --output
            Output stiffness for each nucleosome call in GFF format.
    --range
            Genomic range to consider. Format: [str, All|chr|chr:start-end]  whre 'All' is all genome, 'chr' is a single chomosome, and 'chr:start-end' is the range indicated by the coordinates. Optional, default 'All'.
    --t
            Temperature (K). Optional, default 310.15.

Statistics usage

statistics/nucleR.R

Rscript statistics/nucleR.R --input {gff} --genome {gff} --out_genes {csv} --out_gw {csv}
    --input
            Nucleosome calls in GFF format as obtained from nucleR.
    --genome
            Gene positions in the reference genome. GFF Format.
    --out_genes
            Output file containing statistics of all calculations for each gene. CSV format.
    --out_gw
            Output file containing table of genome wide statistics. CSV format. 

statistics/nucDyn.R

Rscript statistics/nucDyn.R --input {gff} --genome {gff} --out_genes {csv} --out_gw {png}
    --input 
            Nucleosome inclusions, evictions and shifts as obtained from NucDyn. GFF format.
    --genome
            Gene positions in the reference genome. GFF Format.
    --out_genes
            Output file containing statistics of all calculations for each gene. CSV format.
    --out_gw
            Output file containing plot of genome wide statistics. PNG format.

statistics/NFR.R

Rscript statistics/NFR.R --input {gff}  --genome {gff} --out_gw {csv}
    --input
            Nucleosome free regions in GFF format as obtained from NFR analysis.
    --genome 
            Gene positions in the reference genome. GFF Format.
    --out_gw 
            Output file containing table of genome wide statistics. CSV format.

statistics/txstart.R

Rscript statistics/txstart.R --input {gff} --genome {gff} --out_genes {csv} --out_gw {png} --out_gw2 {png}
    --input 
            TSS classification in GFF format as obtained from txstart analysis. 
    --genome
            Gene positions in the reference genome. GFF Format.
    --out_genes
            Output file containing statistics of all calculations for each gene. CSV format.
    --out_gw
            Output file containing table of genome wide statistics. PNG format
    --out_gw2
            Output file containing plot of genome wide statistics. PNG format

statistics/periodicity.R

Rscript statistics/periodicity.R --input {gff} --genome {gff} --out_genes {csv} --out_gw {csv}
    --input 
            Periodicity of genes in GFF format as obtained from periodicity analysis.
    --genome
            Gene positions in the reference genome. GFF Format.
    --out_genes
            Output file containing statistics of all calculations for each gene. CSV format.
    --out_gw
            Output file containing table of genome wide statistics. CSV format.

statistics/stiffness.R

Rscript statistics/stiffness.R -input {gff} --genome {gff} --out_genes {csv} --out_gw {csv} --out_gw2 {png}
    --input 
            Nucleosome calls with estimated stiffness values, in GFF format as obtained from stiffness analysis. 
    --genome
            Gene positions in the reference genome. GFF Format,
    --out_genes
            Output file containing statistics of all calculations for each gene. CSV format.
    --out_gw
            Output file containing table of genome wide statistics. CSV format.
    --out_gw2
            Output file containing plot of genome wide statistics. PNG format.

Results

Most of 'Nucleosome Dynamics CLI' output files are sequence annotation files, either in GFF or BW format. They are ready to be visualized as sequence tracks in most modern sequence browsers. In addition, for each track hit further information is offered to help analysing the rellevance of each individual result. An explanation about each track, and the list of its attributes are explained in the following.

NucDyn

Primary data

  • Position: region where a nucleosome movement is detected.
  • Type: change in the nucleosome map.
  • Score: magnitude of the change.

Attributes

  • class: type of hotspot (see help for all possible types).
  • nreads: number of reads involved in this movement.

nucleR

Primary data

  • Position: region where a nucleosome is detected.
  • Score: Positionning score. It is calculated as the weighted sum of width and height scores.

Attributes

  • score_width: Witdth score. It is a measure peak sharpness. A value of 0 would be an extremely wide peak and a value of 1 a very sharp one.
  • score_height: Height score. It tells how hight a nucleosome peak is. The bigger this number, the higher the peak.
  • class: Whether the nucleosome is well-positioned (W) or fuzzy (F) or undetermined. The class depends on score_h and score_w. Undetermined means the exact position of the nucleosome cannot be determined due to strong fuzziness.

Stiffness

Primary data

  • Score: Apparent stiffness estimation. It represents the energy required to move the nucleosome (expressed in kcal/mol/bp). It's derived from the standard deviation of a fitted Gaussian.

Attributes

  • nucleR_score: the nucleR score given to that nucleosome.
  • nucleR.class: the nucleR class given to that nucleosome.
  • gauss_k: the height of the peak of the gaussian curve.
  • gauss_m: the position of the peak of the gaussian curve.
  • gauss_sd: the standard deviation of the gaussian curve.

Periodicity

Primary data

  • Position: gene position (from TSS to TTS)

Attributes

  • nucleosome_first: Dyad of the first (+1) nucleosome of the gene.
  • nucleosme_last: Dyad of the last (closest to TTS) nucleosome of the gene.
  • score_phase: Ii is a measure of the phase between the first and the last nucleosome. A score of 0 means the two nucleosomes are completely phased and a score close to the nucleosome repeat length of the organism divided by 2 (83 in S. cerevisiae) corresponds to totally antiphased nucleosomes.
  • score_autocorrelation: It is directly computed from the experimental coverage and is a quantitative measure of the periodicity of nucleosomes along the gene body.

TSS classes

Primary data

  • Position: Region between the dyads of two nucleosomes surrounding the TSS.

Attributes

  • classification: Descriptor of the nucleosome architecture around the Transcription Start Site. See the help for possible options.
  • distance: Distance in base pairs between the nucleosome +1 and the nucleosome -1.
  • nucleosome minus1: Position of the nucleosome -1 dyad.
  • nucleosome plus1: Position of the nucleosome +1 dyad.
  • TTS_position: Position of the Transcription Start Site.