1.0.0
). The latest
stable release is
2.1.2
.
Introduction
Nextflow handles job submissions on SLURM or other environments, and supervises running the jobs. Thus the Nextflow process must run until the pipeline is finished. We recommend that you put the process running in the background through screen
/ tmux
or similar tool. Alternatively you can run nextflow within a cluster job submitted your job scheduler.
It is recommended to limit the Nextflow Java virtual machines memory. We recommend adding the following line to your environment (typically in ~/.bashrc
or ~./bash_profile
):
Running the pipeline
The typical command for running the pipeline is as follows:
This will launch the pipeline with the docker
configuration profile. See below for more information about profiles.
Note that the pipeline will create the following files in your working directory:
Updating the pipeline
When you run the above command, Nextflow automatically pulls the pipeline code from GitHub and stores it as a cached version. When running the pipeline after this, it will always use the cached version if available - even if the pipeline has been updated since. To make sure that you’re running the latest version of the pipeline, make sure that you regularly update the cached version of the pipeline:
Reproducibility
It’s a good idea to specify a pipeline version when running the pipeline on your data. This ensures that a specific version of the pipeline code and software are used when you run your pipeline. If you keep using the same tag, you’ll be running the same version of the pipeline, even if there have been changes to the code since.
First, go to the nf-core/atacseq releases page and find the latest version number - numeric only (eg. 1.3.1
). Then specify this when running the pipeline with -r
(one hyphen) - eg. -r 1.3.1
.
This version number will be logged in reports when you run the pipeline, so that you’ll know what you used when you look back in the future.
Main arguments
-profile
Use this parameter to choose a configuration profile. Profiles can give configuration presets for different compute environments. Note that multiple profiles can be loaded, for example: -profile docker
- the order of arguments is important!
If -profile
is not specified at all the pipeline will be run locally and expects all software to be installed and available on the PATH
.
awsbatch
- A generic configuration profile to be used with AWS Batch
conda
docker
- A generic configuration profile to be used with Docker
- Pulls software from dockerhub:
nfcore/atacseq
singularity
- A generic configuration profile to be used with Singularity
- Pulls software from dockerhub:
nfcore/atacseq
test
- A profile with a complete configuration for automated testing
- Includes links to test data so needs no other parameters
--design
You will need to create a design file with information about the samples in your experiment before running the pipeline. Use this parameter to specify its location. It has to be a comma-separated file with 4 columns, and a header row as shown in the examples below.
Multiple replicates
The group
identifier is the same when you have multiple replicates from the same experimental group, just increment the replicate
identifier appropriately. The first replicate value for any given experimental group must be 1. Below is an example for a single experimental group in triplicate:
Multiple runs of the same library
The group
and replicate
identifiers are the same when you have re-sequenced the same sample more than once (e.g. to increase sequencing depth). The pipeline will perform the alignments in parallel, and subsequently merge them before further analysis. Below is an example for two samples sequenced across multiple lanes:
Full design
A final design file may look something like the one below. This is for two experimental groups in triplicate, where the last replicate of the treatment
group has been sequenced twice.
Column | Description |
---|---|
group | Group identifier for sample. This will be identical for replicate samples from the same experimental group. |
replicate | Integer representing replicate number. Must start from 1..<number of replicates> . |
fastq_1 | Full path to FastQ file for read 1. File has to be zipped and have the extension “.fastq.gz” or “.fq.gz”. |
fastq_2 | Full path to FastQ file for read 2. File has to be zipped and have the extension “.fastq.gz” or “.fq.gz”. |
Example design files have been provided with the pipeline for paired-end and single-end data.
Generic arguments
--singleEnd
By default, the pipeline expects paired-end data. If you have single-end data, specify --singleEnd
on the command line when you launch the pipeline.
It is not possible to run a mixture of single-end and paired-end files in one run.
--narrowPeak
MACS2 is run by default with the --broad
flag. Specify this flag to call peaks in narrowPeak mode.
--fragment_size
Number of base pairs to extend single-end reads when creating bigWig files. Default: 0
Reference genomes
The pipeline config files come bundled with paths to the illumina iGenomes reference index files. If running with docker or AWS, the configuration is set up to use the AWS-iGenomes resource.
--genome
(using iGenomes)
There are 31 different species supported in the iGenomes references. To run the pipeline, you must specify which to use with the --genome
flag.
You can find the keys to specify the genomes in the iGenomes config file
. Common genomes that are supported are:
- Human
--genome GRCh37
- Mouse
--genome GRCm38
- Drosophila
--genome BDGP6
- S. cerevisiae
--genome R64-1-1
There are numerous others - check the config file for more.
Note that you can use the same configuration setup to save sets of reference files for your own use, even if they are not part of the iGenomes resource. See the Nextflow documentation for instructions on where to save such a file.
The syntax for this reference configuration is as follows:
--fasta
Full path to fasta file containing reference genome (mandatory if --genome
is not specified). If you don’t have a BWA index available this will be generated for you automatically. Combine with --saveGenomeIndex
to save BWA index for future runs.
--gtf
The full path to GTF file for annotating peaks (mandatory if --genome
is not specified). Note that the GTF file should resemble the Ensembl format.
--bwa_index
Full path to an existing BWA index for your reference genome including the base name for the index.
--gene_bed
The full path to BED file for genome-wide gene intervals. This will be created from the GTF file if it isnt specified.
--tss_bed
The full path to BED file for genome-wide transcription start sites. This will be created from the gene BED file if it isnt specified.
--macs_gsize
Effective genome size parameter required by MACS2. These have been provided when --genome
is set as GRCh37, GRCh38, GRCm38, WBcel235, BDGP6, R64-1-1, EF2, hg38, hg19 and mm10. For other genomes, if this parameter isnt specified then the MACS2 peak-calling and differential analysis will be skipped.
--mito_name
Name of mitochondrial chomosome in reference assembly. Reads aligning to this contig are filtered out if a valid identifier is provided otherwise this step is skipped. Where possible these have been provided in the igenomes.config
.
--blacklist
If provided, alignments that overlap with the regions in this file will be filtered out (see ENCODE blacklists). The file should be in BED format. Blacklisted regions for GRCh37, GRCh38, GRCm38, hg19, hg38, mm10 are bundled with the pipeline in the blacklists
directory, and as such will be automatically used if any of those genomes are specified with the --genome
parameter.
--saveGenomeIndex
If the BWA index is generated by the pipeline use this parameter to save it to your results folder. These can then be used for future pipeline runs, reducing processing times.
--igenomesIgnore
Do not load igenomes.config
when running the pipeline. You may choose this option if you observe clashes between custom parameters and those supplied in igenomes.config
.
Adapter trimming
The pipeline accepts a number of parameters to change how the trimming is done, according to your data type. You can specify custom trimming parameters as follows:
--clip_r1 <NUMBER>
- Instructs Trim Galore to remove bp from the 5’ end of read 1 (for single-end reads).
--clip_r2 <NUMBER>
- Instructs Trim Galore to remove bp from the 5’ end of read 2 (paired-end reads only).
--three_prime_clip_r1 <NUMBER>
- Instructs Trim Galore to remove bp from the 3’ end of read 1 AFTER adapter/quality trimming has been
--three_prime_clip_r2 <NUMBER>
- Instructs Trim Galore to re move bp from the 3’ end of read 2 AFTER adapter/quality trimming has been performed.
--skipTrimming
Skip the adapter trimming step. Use this if your input FastQ files have already been trimmed outside of the workflow or if you’re very confident that there is no adapter contamination in your data.
--saveTrimmed
By default, trimmed FastQ files will not be saved to the results directory. Specify this flag (or set to true in your config file) to copy these files to the results directory when complete.
Alignments
--keepMito
Reads mapping to mitochondrial contig are not filtered from alignments.
--keepDups
Duplicate reads are not filtered from alignments.
--keepMultiMap
Reads mapping to multiple locations in the genome are not filtered from alignments.
--skipMergeReplicates
An additional series of steps are performed by the pipeline by merging the replicates from the same experimental group. This is primarily to increase the sequencing depth in order to perform downstream analyses such as footprinting. Specifying this parameter means that these steps will not be performed.
--saveAlignedIntermediates
By default, intermediate BAM files will not be saved. The final BAM files created after the appropriate filtering step are always saved to limit storage usage. Set to true to also save other intermediate BAM files.
Job resources
Automatic resubmission
Each step in the pipeline has a default set of requirements for number of CPUs, memory and time. For most of the steps in the pipeline, if the job exits with an error code of 143
(exceeded requested resources) it will automatically resubmit with higher requests (2 x original, then 3 x original). If it still fails after three times then the pipeline is stopped.
Custom resource requests
Wherever process-specific requirements are set in the pipeline, the default value can be changed by creating a custom config file. See the files hosted at nf-core/configs
for examples.
If you are likely to be running nf-core
pipelines regularly it may be a good idea to request that your custom config file is uploaded to the nf-core/configs
git repository. Before you do this please can you test that the config file works with your pipeline of choice using the -c
parameter (see definition below). You can then create a pull request to the nf-core/configs
repository with the addition of your config file, associated documentation file (see examples in nf-core/configs/docs
), and amending nfcore_custom.config
to include your custom profile.
If you have any questions or issues please send us a message on Slack.
AWS Batch specific parameters
Running the pipeline on AWS Batch requires a couple of specific parameters to be set according to your AWS Batch configuration. Please use the -awsbatch
profile and then specify all of the following parameters.
--awsqueue
The JobQueue that you intend to use on AWS Batch.
--awsregion
The AWS region to run your job in. Default is set to eu-west-1
but can be adjusted to your needs.
Please make sure to also set the -w/--work-dir
and --outdir
parameters to a S3 storage bucket of your choice - you’ll get an error message notifying you if you didn’t.
Other command line parameters
--outdir
The output directory where the results will be saved.
--email
Set this parameter to your e-mail address to get a summary e-mail with details of the run sent to you when the workflow exits. If set in your user config file (~/.nextflow/config
) then you don’t need to specify this on the command line for every run.
-name
Name for the pipeline run. If not specified, Nextflow will automatically generate a random mnemonic.
This is used in the MultiQC report (if not default) and in the summary HTML / e-mail (always).
NB: Single hyphen (core Nextflow option)
-resume
Specify this when restarting a pipeline. Nextflow will used cached results from any pipeline steps where the inputs are the same, continuing from where it got to previously.
You can also supply a run name to resume a specific run: -resume [run-name]
. Use the nextflow log
command to show previous run names.
NB: Single hyphen (core Nextflow option)
-c
Specify the path to a specific config file (this is a core NextFlow command).
NB: Single hyphen (core Nextflow option) NB: You can use this config to override pipeline defaults.
--custom_config_version
Provide git commit id for custom Institutional configs hosted at nf-core/configs
. This was implemented for reproducibility purposes. Default is set to master
.
--custom_config_base
If you’re running offline, nextflow will not be able to fetch the institutional config files
from the internet. If you don’t need them, then this is not a problem. If you do need them,
you should download the files from the repo and tell nextflow where to find them with the
custom_config_base
option. For example:
Note that the nf-core/tools helper package has a
download
command to download all required pipeline files + singularity containers + institutional configs in one go for you, to make this process easier.
--max_memory
Use to set a top-limit for the default memory requirement for each process.
Should be a string in the format integer-unit. eg. --max_memory '8.GB'
--max_time
Use to set a top-limit for the default time requirement for each process.
Should be a string in the format integer-unit. eg. --max_time '2.h'
--max_cpus
Use to set a top-limit for the default CPU requirement for each process.
Should be a string in the format integer-unit. eg. --max_cpus 1
--plaintext_email
Set to receive plain-text e-mails instead of HTML formatted.
--monochrome_logs
Set to disable colourful command line output and live life in monochrome.
--multiqc_config
Specify a path to a custom MultiQC configuration file.