This pipeline has been deprecated as of June 2018. Please update your pipelines to the official WDL-based ENCODE DCC pipeline at https://github.com/ENCODE-DCC/chip-seq-pipeline2 (June 2018)
June 2018: Note that the updated official ENCODE DCC pipeline is an exact replica of the pipeline in this repository except that it uses WDL instead of BigDataScript for workflow management. We recommend transitioning to the WDL version since it easier to install. Also all future updates and bug fixes will be made to the WDL-based pipeline. If you have processed datasets using the pipeline in this repository, you do NOT need to rerun anything. For future runs, we recommend switching to the WDL-based pipeline.
- Go to Genomic pipelines in Kundaje lab
- Go to Discussion channel
- Jump to Usage
- Jump to Troubleshooting
The AQUAS pipeline implements the ENCODE (phase-3) transcription factor and histone ChIP-seq pipeline specifications (by Anshul Kundaje) in this google doc.
NOTE: We recommend using the WDL-based implementation of this pipeline here as it uses a more stable and maintained workflow management system.
Install software/database in a correct order according to your system. For example on Kundaje lab's clusters, you only need to install one software Pipeline.
-
General computer
-
Kundaje lab's clusters
-
Stanford SCG cluster
-
Stanford Sherlock cluster
Install Java 8 (jdk >= 1.8 or jre >= 1.8) on your system. If you don't have super-user privileges on your system, locally install it and add it to your $PATH
.
-
For Debian/Ubuntu (>14.10) based Linux:
$ sudo apt-get install git openjdk-8-jre
-
For Fedora/Red-Hat based Linux:
$ sudo yum install git java-1.8.0-openjdk
-
For Ubuntu 14.04 (trusty):
$ sudo add-apt-repository ppa:webupd8team/java -y $ sudo apt-get update $ sudo apt-get install oracle-java8-installer
REMOVE ANY ANACONDA OR OTHER VERSIONS OF CONDA FROM YOUR BASH STARTUP SCRIPT. WE CANNOT GUARANTEE THAT PIPELINE WORKS WITH OTHER VERSIONS OF CONDA. ALSO REMOVE R AND OTHER CONFLICTING MODULES FROM IT TOO. Remove any other Anaconda from your $PATH
. Check your loaded modules with $ module list
and unload any Anaconda modules in your bash startup scripts ($HOME/.bashrc
or $HOME/.bash_profile
). Add unset PYTHONPATH
to your bash start up scripts.
Install Miniconda3 latest on your system. IMPORTANT Make sure that the absolute path of the destination directory is short. Long path will cause an error in the depenecies installation step issue #8.
$ wget https://repo.continuum.io/miniconda/Miniconda3-latest-Linux-x86_64.sh
$ bash Miniconda3-latest-Linux-x86_64.sh
Answer yes
for the final question. If you choose no
, you need to manually add Miniconda3 to your $HOME/.bashrc
.
Do you wish the installer to prepend the Miniconda3 install location
to PATH in your /your/home/.bashrc ? [yes|no]
[no] >>> yes
Open a new terminal after installation.
Install BigDataScript v0.99999e (forked) on your system. The original BDS v0.99999e does not work correctly with the pipeline (see PR #142 and issue #131).
$ wget https://github.com/leepc12/BigDataScript/blob/master/distro/bds_Linux.tgz?raw=true -O bds_Linux.tgz
$ mv bds_Linux.tgz $HOME && cd $HOME && tar zxvf bds_Linux.tgz
Add export PATH=$PATH:$HOME/.bds
to your $HOME/.bashrc
. If Java memory occurs, add export _JAVA_OPTIONS="-Xms256M -Xmx728M -XX:ParallelGCThreads=1"
too.
Get the latest version of the pipeline.
$ git clone https://github.com/kundajelab/TF_chipseq_pipeline
Install software dependencies automatically. It will create two conda environments (aquas_chipseq and aquas_chipseq_py3) under your conda.
$ bash install_dependencies.sh
If you don't use install_dependencies.sh
, manually replace BDS's default bds.config
with a correct one:
$ cp bds.config ./utils/bds_scr $HOME/.bds
If install_dependencies.sh
fails, run ./uninstall_dependencies.sh
, fix problems and then try bash install_dependencies.sh
again.
Install genome data for a specific genome [GENOME]
. Currently hg19
, mm9
, hg38
and mm10
are available. Specify a directory [DATA_DIR]
to download genome data. A species file generated on [DATA_DIR]
will be automatically added to your ./default.env
so that the pipeline knows that you have installed genome data using install_genome_data.sh
. If you want to install multiple genomes make sure that you use the same directory [DATA_DIR]
for them. Each genome data will be installed on [DATA_DIR]/[GENOME]
. If you use other BDS pipelines, it is recommended to use the same directory [DATA_DIR]
to save disk space.
IMPORTANT: install_genome_data.sh
can take longer than an hour for downloading data and building index. DO NOT run the script on a login node, use qlogin
for SGE and srun --pty bash
for SLURM.
# DO NOT run this on a login node
$ bash install_genome_data.sh [GENOME] [DATA_DIR]
If you have super-user privileges on your system, it is recommended to install genome data on /your/data/bds_pipeline_genome_data
and share them with others.
$ sudo su
$ bash install_genome_data.sh [GENOME] /your/data/bds_pipeline_genome_data
You can find a species file [SPECIES_FILE]
on /your/data/bds_pipeline_genome_data
for each pipeline type. Then others can use the genome data by adding -species_file [SPECIES_FILE_PATH]
to the pipeline command line. Or they need to add species_file = [SPECIES_FILE_PATH]
to the section [default]
in their ./default.env
.
AQUAS pipeline does not need internet connection but installers (install_dependencies.sh
and install_genome_data.sh
) do need it. So the workaround should be that first install dependencies and genome data on a computer that is connected to the internet and then move Conda and genome database directories to your internet-free one. Both computers should have THE SAME LINUX VERSION.
-
On your computer that has an internet access,
- Follow the installation instruction for general computers
- Move your Miniconda3 directory to
$HOME/miniconda3
on your internet-free computer. - Move your genome database directory, which has
aquas_chipseq_species.conf
and directories per species, to$HOME/genome_data
on your internet-free computer.$HOME/genome_data
on your internet-free computer should haveaquas_chipseq_species.conf
. - Move your BDS directory
$HOME/.bds
to$HOME/.bds
on your internet-free computer. - Move your pipeline directory
chipseq_pipelines/
to$HOME/chipseq_pipelines/
on your internet-free computer.
-
On your internet-free computer,
-
Add your
miniconda3/bin
and BDS binary to$PATH
in your bash initialization script ($HOME/.bashrc
or$HOME/.bash_profile
).export PATH="$PATH:$HOME/miniconda3/bin" export PATH="$PATH:$HOME/.bds"
-
Modify
[default]
section in$HOME/chipseq_pipelines/default.env
.[default] conda_bin_dir=$HOME/miniconda3/bin species_file=$HOME/genome_data/aquas_chipseq_species.conf
-
-
Modify all paths in
$HOME/genome_data/aquas_chipseq_species.conf
so that they correctly point to the right files. -
Check BDS version.
$ bds -version Bds 0.99999e (build 2016-08-26 06:34), by Pablo Cingolani
-
Make sure that your java rumtime version is >= 1.8.
$ java -version java version "1.8.0_111" Java(TM) SE Runtime Environment (build 1.8.0_111-b14) Java HotSpot(TM) 64-Bit Server VM (build 25.111-b14, mixed mode)
We recommend using BASH to run pipelines.
IMPORTANT! The latest version of the pipeline includes a Python wrapper chipseq.py
to parse command line arguments and JSON configuration file. python chipseq.py
takes the same command line arguments as in the original bds chipseq.bds
. However, chipseq.py
takes in JSON configuration file instead of the original INI one.
There are two ways to define parameters for ChIP-Seq pipelines. Default values for most of those parameters are already given. Take a look at example commands and configuration files in examples. AQUAS pipeline is multi-threaded. Set up maximum number of processors with -nth
.
-
Parameters from command line arguments: Any of three positional arguments can be skipped. Then default values will be used for skipped ones. Choose
[CHIPSEQ_TYPE]
betweenTF
(default) andhistone
. You can also specify it with-type [CHIPSEQ_TYPE]
. You can stop the pipeline at the end of any stage. Choose[FINAL_STAGE]
amongbam
,filt_bam
,tag
,xcor
,peak
andidr
(default). You can also specify it with-final_stage [FINAL_STAGE]
. See Pipeline steps for details about pipeline stages.$ python chipseq.py [CHIPSEQ_TYPE] [FINAL_STAGE] [CONF_JSON_FILE] -species [SPECIES] -nth [NUM_THREADS] -fastq1 ... -fastq2 ... -ctl_fastq1 ...
-
Parameters from a configuration JSON file: Note that both command line arguments and a configruation JSON share the same key name. In a configuration JSON, only the deepest keys and values are taken. Any JSON structure/hierachy to group those keys is allowed. See full example JSON and reduced example JSON how to group keys.
$ python chipseq.py [CONF_JSON_FILE] # CONF_JSON_FILE (can work without group hierachy) { "type" : "[CHIPSEQ_TYPE]", "final_stage" : "[FINAL_STAGE]" "fastq1" : "...", "fastq2" : "...", "ctl_fastq1" : "...", ... "species" : "hg19", "nth" : [NUM_THREADS] }
-
You can mix up method 1 and 2. Parameters specied in command line arguments will override the other.
To list all parameters: $ python chipseq.py -h
Press Ctrl + C on a terminal or send any kind of kill signals to it. Please note that this will delete all intermediate files and incomplete outputs for the running tasks. AQUAS pipeline automatically determines if each task has finished or not (by comparing timestamps of input/output files for each task). To run the pipeline from the point of failure, correct error first and then just run the pipeline with the same command that you started the pipeline with. There is no additional parameter for restarting the pipeline.
On servers with a cluster engine (such as Sun Grid Engine and SLURM), DO NOT QSUB/SBATCH BDS COMMAND LINE. Run BDS command directly on login nodes. BDS is a task manager and it will automatically submit(qsub/sbatch) and manage its sub tasks. You can choose [CLUSTER_ENGINE]
between sge
(default on Kundaje), slurm
(default on Sherlock and SCG) and local
(default for others). You can also let BDS submit its subtasks to a specific queue/partition [QUEUE_NAME]
on Sun Grid Engine or SLURM.
$ python chipseq.py -system sge -q [SGE_QUEUE_NAME] ...
$ python chipseq.py -system slurm -q [SLURM_PARTITON_NAME] ... # Sherlock example
$ python chipseq.py -system slurm -q_for_slurm_account -q [SLURM_ACCOUNT_NAME] ... # SCG example
IMPORTANT! Please read this section carefully if you run pipelines on Stanford SCG and Sherlock cluster.
Most clusters have a policy to limit number of threads and memory per user on a login node. One BDS process, as a Java-based task manager, takes up to 1GB of memory and 50 threads even though it just submits/monitors subtasks. So if you want to run more than 50 pipelines in parallel, your cluster will kill BDS processes due to resource limit on a login node (check resource limit per user with ulimit -a
). For example of 50 pipelines, 50 GB of memory and 2500 threads will be taken by 50 BDS processes. So the Workaround for this is to make an interactive node to keep all BDS processes alive. Such interactive node must have long walltime enough to wait for all pipelines in it to finish. Recommended resource setting is 1.0GB memory per pipeline.
SGE example to make an interactive node for 100 pipelines: 1 cpu, 100GB memory, 3 days walltime.
$ qlogin -l h_rt=72:00:00 -l h_vmem=100G
SLURM example to make an interactive node for 100 pipelines: 1 cpu, 100GB memory, 3 days walltime.
$ srun -n 1 --mem 100G -t 3-0 -p [YOUR_PARTITON] --qos normal --pty /bin/bash -i -l
$ srun -n 1 --mem 100G -t 3-0 --account [YOUR_ACCOUNT] --qos normal --pty /bin/bash -i -l
Once you get an interactive node, repeat the following commands per sample to run a pipeline.
$ cd [WORK_DIR]
$ python chipseq.py -screen [SCREEN_NAME] -system [CLUSTER_ENGINE: slurm or sge] -q [SGE_QUEUE_OR_SLURM_PARTITION] -nth [MAX_NUM_THREAD_PER_PIPELINE] ...
$ python chipseq.py -screen [SCREEN_NAME] -system slurm -q_for_slurm_account -q [SLURM_ACCOUNT] -nth [MAX_NUM_THREAD_PER_PIPELINE] ...
$ sleep 2 # wait for 2 seconds for safety
Then you can monitor your pipelines with screen -ls
and tail -f [WORK_DIR]/[SCREEN_NAME].BSD.log
. If you want to run more than 200 pipelines, you would want to make multiple interactive nodes and distribute your samples to them.
There are five data types; fastq
, bam
, filt_bam
, tag
and peak
.
- For exp. replicates: define data path with
-[DATA_TYPE][REPLICATE_ID]
. - For contols: define data path with
-ctl_[DATA_TYPE][CONTROL_ID]
.
You can skip [REPLICATE_ID]
or [CONTROL_ID]
if it's 1. (eg. -fastq
, -ctl_bam
, -tag
, ... ). Except for fastq, add -pe
if your data set is PAIRED-END. You can also individually specify endedness for each replicate; -pe[REPLICATE_ID]
for exp. replicates, -ctl_pe[CONTROL_ID]
for controls.
-
Starting from fastqs: see the example in the previous section
-
Starting from paired end bams:
$ python chipseq.py -species hg19 -pe -bam1 /DATA/REP1.bam -bam2 /DATA/REP2.bam -ctl_bam /DATA/CTL.bam ...
-
Starting from singled-ended deduped / filtered bams:
$ python chipseq.py -species hg19 -se -filt_bam1 /DATA/REP1.filt.bam -filt_bam2 /DATA/REP2.filt.bam -ctl_filt_bam /DATA/CTL.filt.bam ...
-
Starting from paired end tagaligns:
$ python chipseq.py -species mm9 -pe -tag1 /DATA/REP1.tagAlign.gz -tag2 /DATA/REP2.tagAlign.gz -ctl_tag /DATA/CTL.tagAlign.gz
-
Starting from narrow/relaxed(region) peak files:
$ python chipseq.py -species hg19 -peak1 /DATA/Example1.regionPeak.gz -peak2 /DATA/Example2.regionPeak.gz -peak_pooled /DATA/Example.pooled.regionPeak.gz ...
If you want do perform full IDR including pseudo-replicates and pooled pseudo-replicates, add the following to the command line.
- For IDR on pseduro replicates of replicate 1:
-peak1_pr1 [PEAK1_PR1] -peak1_pr2 [PEAK1_PR2]
- For IDR on pseduro replicates of replicate 2:
-peak2_pr1 [PEAK2_PR1] -peak2_pr2 [PEAK2_PR2]
- For IDR on pseduro replicates of replicate N:
-peakN_pr1 [PEAK2_PR1] -peakN_pr2 [PEAK2_PR2]
- For IDR on pooled pseduro replicates:
-peak_ppr1 [PEAK_PPR1] -peak_ppr2 [PEAK_PPR2]
- For IDR on pseduro replicates of replicate 1:
-
Mixing up input types:
$ python chipseq.py -species mm9 -se -fastq1 /DATA/REP1.fastq.gz -bam2 /DATA/ENCSR000EGM/REP2.bam -ctl_tag /DATA/CTL.tagAlign.gz
All data are treated as SINGLED-ENDED if endedness is not explicltly specifed. Endedness is automatically detected for fastqs.
Add -pe
to the command line if all data set are paired-end. You can also individually specify endedness for each replicate.
- For exp. replicates:
-pe[REPLICATE_ID]
- For controls:
-ctl_pe[CONTROL_ID]
For fastqs, you do not need to add '-pe' since the pipeline will automatically determine it according to indices in command line parameters.
-
For exp. replicates:
- Define data path as -fastq[REPLICATE_ID], then it's SE (single ended).
- Define data path as -fastq[REPLICATE_ID]_[PAIRING_ID], then it's PE.
-
For controls:
- Define data path as -ctl_fastq[REPLICATE_ID], it's SE.
- Define data path as -ctl_fastq[REPLICATE_ID]_[PAIRING_ID], it's PE.
-
Example: 2 replicates and 1 control replicate (all SE)
$ python chipseq.py -species hg19 -fastq1 /DATA/REP1.fastq.gz -fastq2 /DATA/REP2.fastq.gz -ctl_fastq1 /DATA/CTL.fastq.gz
-
Example: 2 replicates and 2 control replicates (all PE)
$ python chipseq.py -species hg19 -fastq1_1 /DATA/REP1_1.fastq.gz -fastq1_2 /DATA/REP1_2.fastq.gz -fastq2_1 /DATA/REP2_1.fastq.gz -fastq2_2 /DATA/REP2_2.fastq.gz -ctl_fastq1_1 /DATA/Ctl/CTL_1_1.fastq.gz -ctl_fastq1_2 /DATA/Ctl/CTL_1_2.fastq.gz -ctl_fastq2_1 /DATA/Ctl/CTL_2_1.fastq.gz -ctl_fastq2_2 /DATA/Ctl/CTL_2_1.fastq.gz
You can mix up not only data types but also endedness.
-
Example: 1 SE fastq, 1 PE bam and 1 PE control tagalign
$ python chipseq.py -species hg19 -fastq1 /DATA/REP1.fastq.gz -pe2 -bam2 /DATA/REP2.bam -pe_ctl -ctl_tag /DATA/CTL.tagAlign.gz
AQUAS pipeline goes through the following stages:
- bam : mapping (fastq -> bam)
- filt_bam : filtering and deduping bam (bam -> filt_bam)
- tag : creating tagalign (filt_bam -> tagalign)
- xcor : cross-correlation analysis (tagalign -> xcor plot.pdf/score.txt )
- peak : peak calling (tagalign -> peak)
- idr : IDR (peaks -> IDR score and peaks)
AQUAS pipeline stops right after -final_stage [STAGE]
(idr
by default). It is useful if you are not interested in peak calling and want to map/align lots of genome data (fastq, bam or filt_bam) IN PARALLEL.
For completely serialized jobs, add -no_par
to the command line. Individual tasks can still go multi-threaded.
IMPORTANT! You can set up a limit for total number of threads with -nth [MAX_TOTAL_NO_THREADS]
. Total number of threads used by a pipeline will not exceed this limit.
Default -nth
for each cluster is defined on ./default.env
(e.g. 16 on SCG and 8 on Kundaje lab cluster)
The pipeline automatically distributes [MAX_TOTAL_NO_THREADS]
threads for jobs according to corresponding input file sizes. For example of two fastqs (1GB and 2GB) with -nth 6
, 2 and 4 threads are allocated for aligning 1GB and 2GB fastqs, respectively. The same policy applies to other multi-threaded tasks like deduping and peak calling.
However, all multi-threaded tasks (like bwa, bowtie2, spp and macs2) still have their own max. memory (-mem_APPNAME [MEM_APP]
) and walltime (-wt_APPNAME [WALLTIME_APP]
) settings. Max. memory is NOT PER CPU. For example on Kundaje lab cluster (with SGE flag activated bds -s sge chipseq.bds ...
), the actual shell command submitted by BDS for each task is like the following:
qsub -V -pe shm [NTH_ALLOCATED_FOR_APP] -h_vmem=[MEM_APP]/[NTH_ALLOCATED_FOR_APP] -h_rt=[WALLTIME_APP] -s_rt=[WALLTIME_APP] ...
This ensures that total memory reserved for a cluster job equals to [MEM_APP]
. The same policy applies to SLURM.
There are two peak callers (spp
and macs2
) supported by the pipeline. spp
and macs2
are by default for TF ChIP-seq and histone ChIP-seq, respectively. But you can specify a peak caller regardless of the [CHIPSEQ_TYPE]. Simply add -peak_caller [PEAK_CALLER_FOR_IDR]
to the command line.
There are two dup markers (picard
and sambamba
) supported by the pipeline. picard
is by default. picard
is based on Java so there can be a lot Java-related issues (e.g. Java heap error). To change the dup marker to sambamba
, simply add -dup_marker sambamba
to the command line.
Simply add -screen [SCREEN_NAME]
to create a detached screen for a pipeline and then stdout/stderr will be redirected to a log file [SCREEN_NAME].log
. If a log file already exists, stdout/stderr will be appended to it. Monitor the pipeline with tail -f [SCREEN_NAME].log
. A screen will be automatically closed once the pipeline run is done. To kill a pipeline manually while it's running, use ./utils/kill_scr
or screen -X quit
:
$ screen -X -S [SCREEN_NAME] quit
$ kill_scr [SCREEN_NAME]
Picard tools is used for marking dupes in the reads and it's based on Java. If you see any Java heap space errors then increase memory limit for Java with -mem_dedup [MEM]
(default: 12G
).
If your /tmp
quickly fills up and you want to change temporary directory for all Java apps in the pipeline, then add the following line to your bash startup script ($HOME/.bashrc
). Our pipeline takes in $TMPDIR
(not $TMP
) for all Java apps.
export TMPDIR=/your/temp/dir/
Another quick workaround for dealing with Java issues is not to use Picard tools in the pipeline. Add -use_sambamba_markdup
to your command line and then you can use sambamba markdup
instead of picard markdup
.
Please refer to the section Installer for genome data
on BDS pipeline programming.
For general use, use the following command line. You can skip first three positional arguments to use default values.
$ python chipseq.py [CHIPSEQ_TYPE; TF(default), histone] [FINAL_STAGE: bam, filt_bam, tag, xcor, peak, idr(default)] [CONF_JSON_FILE] -species [SPECIES; hg19, mm9, ... ] -nth [NUM_THREADS] -fastq1 [READ_REP1] -fastq2 [READ_REP2] ...
IMPORTANT! If your data set is PAIRED END add the following to the command line, otherwise the pipeline works for SE by default.
-pe
You can also individually specify endedness for each replicate.
-se[REPLICATE_ID] # for exp. replicates,
-se1 -pe2 -se3 ...
If you have just one replicate (PE), define fastqs with -fastq[REP_ID]_[PAIR_ID]
.
-fastq1_1 [READ_PAIR1] -fastq1_2 [READ_PAIR2] \
For multiple replicates (PE), define fastqs with -fastq[REP_ID]_[PAIR_ID]
. Add -fastq[]_[]
for each replicate and pair to the command line:replicates.
-fastq1_1 [READ_REP1_PAIR1] -fastq1_2 [READ_REP1_PAIR2] -fastq2_1 [READ_REP2_PAIR1] -fastq2_2 [READ_REP2_PAIR2] ...
For multiple replicates (SE), define fastqs with -fastq[REP_ID]
:
-se -fastq1 [READ_REP1] -fastq2 [READ_REP2] ...
You can start from bam files. There are two kinds of bam files (raw or deduped) and you need to explicitly choose between raw bam (bam) and deduped one (filt_bam). Don't forget to add -pe
if they are paired end (PE). For raw bams,
-bam1 [RAW_BAM_REP1] -bam2 [RWA_BAM_REP1] ...
For deduped (filtered) bams:
-filt_bam1 [FILT_BAM_REP1] -filt_bam2 [FILT_BAM_REP1] ...
For tagaligns (non-tn5-shifted):
-tag1 [TAGALIGN_REP1] -tag2 [TAGALIGN_REP2] ...
You can also mix up any data types.
-bam1 [RAW_BAM_REP1] -tag2 [TAGALIGN_REP2] ...
For controls, simply add a prefix ctl_
to the parameters. This rule applies to the endedness of controls too. You can also have multiple sets of controls. For example of 2 PE controls,
-ctl_pe -ctl_fastq1_1 [FASTQ_CTL1_PAIR1] -ctl_fastq1_2 [FASTQ_CTL1_PAIR2] -ctl_fastq2_1 [FASTQ_CTL1_PAIR1] -ctl_fastq2_2 [FASTQ_CTL1_PAIR2] ...
If your control is raw bam (paired end).
-ctl_pe -ctl_bam1 [BAM_CTL1] ...
To subsample beds (tagaligns) add the following to the command line. This is different from subsampling for cross-corr. analysis. Peaks will be called with subsampled tagaligns.
-subsample_chip [NO_READS_TO_SUBSAMPLE]
To subsample control beds (tagaligns) add the following to the command line.
-subsample_ctl [NO_READS_TO_SUBSAMPLE]
To change # of lines to subsample for cross-corr. analysis. This will not affect tasks downstream (peak calling and IDR).
-subsample_xcor [NO_READS_TO_SUBSAMPLE]
To disable pseudo replicate generation, add the following. By default, peak calling and IDR will be done for true replicates and pseudo replicates, but if you have -true_rep
in the command line, you will also get IDR on true replicates only.
-true_rep
-true_rep
disables peak calling for pooled replicates as well as self pseudo replicates. If you want to call peaks on true/pooled replicates:
-no_pseudo_rep
You can change the IDR threshold.
-idr_thresh [IDR_THRESHOLD]
You can specify a peak caller for IDR regardless of the type of ChIP-seq.
-peak_caller [PEAK_CALLER; spp, macs2]
To disable cross-corr. analysis.
-no_xcor
If you turn off cross-corr. analysis (-no_xcor
) make sure to set both -extsize_macs2 [EXTSIZE]
and -speak_spp [SPEAK]
. Those two values are supposed to be taken from cross-corr. analysis.
There are two kinds of HTML reports provided by the pipeline.
-
BigDataScript HTML report for debugging: Located at the working folder with name chipseq_[TIMESTAMP]_report.html. This report is automatically generated by BigDataScript and is useful for debugging since it shows summary, timeline, Stdout and Stderr for each job.
-
ChIP-Seq pipeline report for QC and result: The pipeline automatically generate a nice HTML report (Report.html) on its output directory (specified with -out_dir or just './out'). It summarizes files and directory structure, includes QC reports and show a workflow diagram and genome browser tracks for peaks and signals (bigwigs for pValue and fold change). Move your output directory to a web directory (for example, /var/www/somewhere) or make a softlink of it to a web directory. For genome browser tracks, specify your web directory root for your output While keeping its structure. Make sure that you have bgzip and tabix installed on your system. Add the following to the command line:
-url_base http://your/url/to/output -title [PREFIX_FOR_YOUR_REPORT]
If you stop a BDS pipeline with Ctrl+C
while calling peaks with spp
. Temporary files generated by Rscript
are not removed and they are still on $TMP
(or /tmp
if not explicitly exported). You need to manually remove them.
For more details, refer to the file table section in an HTML report generated by the pipeline.
out # root dir. of outputs
│
├ *report.html # HTML report
├ *tracks.json # Tracks datahub (JSON) for WashU browser
├ ENCODE_summary.json # Metadata of all datafiles and QC results
│
├ align # mapped alignments
│ ├ rep1 # for true replicate 1
│ │ ├ *.bam # raw bam
│ │ ├ *.nodup.bam # filtered and deduped bam
│ │ ├ *.tagAlign.gz # tagAlign (bed6) generated from filtered bam
│ │ ├ *.*M.tagAlign.gz # subsampled tagAlign for cross-corr. analysis
│ ├ rep2 # for true repilicate 2
│ ...
│ ├ ctl1 # for control 1
│ ...
│ ├ pooled_rep # for pooled replicate
│ ├ pseudo_reps # for self pseudo replicates
│ │ ├ rep1 # for replicate 1
│ │ │ ├ pr1 # for self pseudo replicate 1 of replicate 1
│ │ │ └ pr2 # for self pseudo replicate 2 of replicate 1
│ │ ├ rep2 # for repilicate 2
│ │ ...
│ └ pooled_pseudo_reps # for pooled pseudo replicates
│ ├ ppr1 # for pooled pseudo replicate 1 (rep1-pr1 + rep2-pr1 + ...)
│ └ ppr2 # for pooled pseudo replicate 2 (rep1-pr2 + rep2-pr2 + ...)
│
├ peak # peaks called
│ ├ macs2 # peaks generated by MACS2
│ │ ├ rep1 # for replicate 1
│ │ │ ├ *.narrowPeak.gz # narrowPeak
│ │ │ ├ *.gappedPeak.gz # gappedPeak
│ │ │ ├ *.filt.narrowPeak.gz # blacklist filtered narrowPeak
│ │ │ ├ *.filt.gappedPeak.gz # blacklist filtered gappedPeak
│ │ ├ rep2 # for replicate 2
│ │ ...
│ │ ├ pseudo_reps # for self pseudo replicates
│ │ └ pooled_pseudo_reps # for pooled pseudo replicates
│ │
│ ├ spp # peaks generated by SPP
│ │ ├ rep1 # for replicate 1
│ │ │ ├ *.regionPeak.gz # regionPeak (narrowPeak format) generated from SPP
│ │ │ ├ *.filt.regionPeak.gz # blacklist filtered narrowPeak
│ │ ├ rep2 # for replicate 2
│ │ ...
│ │ ├ pseudo_reps # for self pseudo replicates
│ │ └ pooled_pseudo_reps # for pooled pseudo replicates
│ │
│ └ idr # IDR thresholded peaks (using peaks from SPP)
│ ├ true_reps # for replicate 1
│ │ ├ *.narrowPeak.gz # IDR thresholded narrowPeak
│ │ ├ *.filt.narrowPeak.gz # IDR thresholded narrowPeak (blacklist filtered)
│ │ └ *.12-col.bed.gz # IDR thresholded narrowPeak track for WashU browser
│ ├ pseudo_reps # for self pseudo replicates
│ │ ├ rep1 # for replicate 1
│ │ ...
│ ├ optimal_set # optimal IDR thresholded peaks
│ │ └ *.filt.narrowPeak.gz # IDR thresholded narrowPeak (blacklist filtered)
│ ├ conservative_set # optimal IDR thresholded peaks
│ │ └ *.filt.narrowPeak.gz # IDR thresholded narrowPeak (blacklist filtered)
│ ├ pseudo_reps # for self pseudo replicates
│ └ pooled_pseudo_reps # for pooled pseudo replicate
│
├ qc # QC logs
│ ├ *IDR_final.qc # Final IDR QC
│ ├ rep1 # for true replicate 1
│ │ ├ *.flagstat.qc # Flagstat QC for raw bam
│ │ ├ *.dup.qc # Picard (or sambamba) MarkDuplicate QC log
│ │ ├ *.pbc.qc # PBC QC
│ │ ├ *.nodup.flagstat.qc # Flagstat QC for filtered bam
│ │ ├ *M.cc.qc # Cross-correlation analysis score for tagAlign
│ │ └ *M.cc.plot.pdf/png # Cross-correlation analysis plot for tagAlign
│ ...
│
├ signal # signal tracks
│ ├ macs2 # signal tracks generated by MACS2
│ │ ├ rep1 # for true replicate 1
│ │ │ ├ *.pval.signal.bigwig (E) # signal track for p-val
│ │ │ └ *.fc.signal.bigwig (E) # signal track for fold change
│ ...
│ └ pooled_rep # for pooled replicate
│
└ report # files for HTML report
For each pipeline rune, ENCODE_summary.json
file is generated under the output directory (-out_dir
). This JSON file includes all metadata and QC metrics.
./utils/parse_summary_qc_recursively.py
recursively finds ENCODE_summary.json
files and parse them to generate one big TSV spreadsheet for QC metrics.
$ python parse_summary_qc_recursively.py -h
usage: ENCODE_summary.json parser for QC [-h] [--out-file OUT_FILE]
[--search-dir SEARCH_DIR]
[--json-file JSON_FILE]
Recursively find ENCODE_summary.json, parse it and make a TSV spreadsheet of
QC metrics.
optional arguments:
-h, --help show this help message and exit
--out-file OUT_FILE Output TSV filename)
--search-dir SEARCH_DIR
Root directory to search for ENCODE_summary.json
--json-file JSON_FILE
Specify json file name to be parsed
-
For python2 (python 2.x >= 2.7) and R-3.x, requirements.txt
-
For python3, requirements_py3.txt
See more troubleshootings.
Example:
[bwa_aln] 17bp reads: max_diff = 2
[bwa_aln] 38bp reads: max_diff = 3
[bwa_aln] 64bp reads: max_diff = 4
[bwa_aln] 93bp reads: max_diff = 5
[bwa_aln] 124bp reads: max_diff = 6
[bwa_aln] 157bp reads: max_diff = 7
[bwa_aln] 190bp reads: max_diff = 8
[bwa_aln] 225bp reads: max_diff = 9
[bwa_read_seq] 0.2% bases are trimmed.
[bwa_aln_core] calculate SA coordinate... 21.39 sec
[bwa_aln_core] write to the disk... 0.10 sec
[bwa_aln_core] 262144 sequences have been processed.
[bwa_read_seq] 0.2% bases are trimmed.
[bwa_aln_core] calculate SA coordinate... 21.27 sec
[bwa_aln_core] write to the disk... 0.09 sec
[bwa_aln_core] 524288 sequences have been processed.
[bwa_read_seq] 0.2% bases are trimmed.
[bwa_aln_core] calculate SA coordinate... 21.51 sec
[bwa_aln_core] write to the disk... 0.08 sec
[bwa_aln_core] 786432 sequences have been processed.
[bwa_read_seq] 0.2% bases are trimmed.
[bwa_aln_core] calculate SA coordinate... 21.34 sec
[bwa_aln_core] write to the disk... 0.08 sec
[bwa_aln_core] 1048576 sequences have been processed.
[bwa_read_seq] 0.2% bases are trimmed.
[bwa_aln_core] calculate SA coordinate... 21.83 sec
[bwa_aln_core] write to the disk... 0.07 sec
[bwa_aln_core] 1309550 sequences have been processed.
[gzclose] buffer error
Solution1 (BEST): Use bwa-0.7.3 or bwa-0.6.2.
$ git clone https://github.com/lh3/bwa bwa-0.7.3
$ cd bwa-0.7.3
$ git checkout tags/0.7.3
$ make
$ ./bwa
Then, append -addpath /path/to/your/bwa
to your command line.
Solution2: Upgrade zlib to 1.2.8
$ BWA_VER=0.7.3
$ git clone https://github.com/lh3/bwa
$ cd bwa
$ git checkout tags/${BWA_VER}
$ sed -e's#INCLUDES=#INCLUDES=-Izlib-1.2.8/ #' -e's#-lz#zlib-1.2.8/libz.a#' Makefile > Makefile.zlib
$ make clean
$ wget http://zlib.net/zlib-1.2.8.tar.gz
$ tar xvzf zlib-1.2.8.tar.gz
$ cd zlib-1.2.8
$ ./configure
$ make
$ cd ..
$ make -f Makefile.zlib
$ ./bwa
Tested bwa versions (with zlib 1.2.8)
- successful: 0.6.2 0.7.1 0.7.2 0.7.3
- failed: 0.7.4 0.7.5 0.7.7 0.7.8 0.7.11 0.7.12
An example of a failed job due to lack of memory (desktop with 4 cores and 12 GB of memory):
[bam_header_read] EOF marker is absent. The input is probably truncated.
[bwa_read_seq] 0.0% bases are trimmed.
[bwa_aln_core] convert to sequence coordinate... [bwt_restore_sa] Failed to allocate 1547846992 bytes at bwt.c line 404: Cannot allocate memory
[samopen] SAM header is present: 25 sequences.
[sam_read1] reference 'ID:bwa PN:bwa VN:0.7.3-r789 CL:bwa samse /home/leepc12/run/index/encodeHg19Male_bwa-0.7.3.fa /home/leepc12/run/ENCSR000EGM3/out/TEST_Rep2.sai /home/leepc12/run/ENCODE/ENCFF000YLY.fastq.gz
' is recognized as '*'.
[main_samview] truncated file.
Solution: balance memory usage between parallel jobs or disable parallel jobs (add '-no_par')
$ python chipseq.py -no_par ...
For computers with limited memory, bwa samse/sampe fails without non-zero exit value. This leads to a failure of a pipeline or corruption of outputs.
Solution: balance memory usage between parallel jobs or disable parallel jobs (add '-no_par')
$ python chipseq.py -no_par ...
Unload any Anaconda Python modules. Remove locally installed Anaconda Python from your $PATH
Warning message:
In min(npld$y[npld$fdr <= fdr]) :
no non-missing arguments to min; returning Inf
excluding systematic background anomalies ... done
calculating statistical thresholds
FDR 0.99 threshold= Inf
Detected 0 peaks
Check if number of reads in your control tagalign is too high, and then reduce it with -subsample_ctl [NO_READ_TO_SUBSAMPLE_CONTROL]
.
Try with half of the original number of reads in control.
- Jin wook Lee - PhD Student, Mechanical Engineering Dept., Stanford University
- Nathan Boley - Postdoc, Dept. of Genetics, Stanford University
- Anshul Kundaje - Assistant Professor, Dept. of Genetics, Stanford University