nf-core/viralrecon
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Assembly and intrahost/low-frequency variant calling for viral samples

ampliconarticassemblycovid-19covid19illuminalong-read-sequencingmetagenomicsnanoporeontoxford-nanoporesars-cov-2variant-callingviralvirus

Launch version 2.6.0 https://github.com/nf-core/viralrecon

Pipeline parameters

Please provide pipeline parameters via the CLI or Nextflow -params-file option. Custom config files including those provided by the -c Nextflow option can be used to provide any configuration except for parameters; see docs.

Samplesheet format

Illumina

You will need to create a samplesheet with information about the samples you would like to analyse before running the pipeline. Use this parameter to specify its location. It has to be a comma-separated file with 3 columns, and a header row as shown in the examples below.

--input '[path to samplesheet file]'

The sample identifiers have to be the same when you have re-sequenced the same sample more than once (e.g. to increase sequencing depth). The pipeline will concatenate the raw reads before performing any downstream analysis.

A final samplesheet file may look something like the one below. SAMPLE_1 was sequenced twice in Illumina PE format, SAMPLE_2 was sequenced once in Illumina SE format.

sample,fastq_1,fastq_2
SAMPLE_1,AEG588A1_S1_L002_R1_001.fastq.gz,AEG588A1_S1_L002_R2_001.fastq.gz
SAMPLE_1,AEG588A1_S1_L003_R1_001.fastq.gz,AEG588A1_S1_L003_R2_001.fastq.gz
SAMPLE_2,AEG588A2_S4_L003_R1_001.fastq.gz,

Column	Description
`sample`	Custom sample name. This entry will be identical for multiple sequencing libraries/runs from the same sample.
`fastq_1`	Full path to FastQ file for Illumina short reads 1. File has to be gzipped and have the extension “.fastq.gz” or “.fq.gz”.
`fastq_2`	Full path to FastQ file for Illumina short reads 2. File has to be gzipped and have the extension “.fastq.gz” or “.fq.gz”.

NB: Dashes (-) and spaces in sample names are automatically converted to underscores (_) to avoid downstream issues in the pipeline.

Nanopore

You have the option to provide a samplesheet to the pipeline that maps sample ids to barcode ids. This allows you to associate barcode ids to clinical/public database identifiers that can be used to QC or pre-process the data with more appropriate sample names.

--input '[path to samplesheet file]'

It has to be a comma-separated file with 2 columns. A final samplesheet file may look something like the one below:

sample,barcode
21X983255,1
70H209408,2
49Y807476,3
70N209581,4

Column	Description
`sample`	Custom sample name, one per barcode.
`barcode`	Barcode identifier attributed to that sample during multiplexing. Must be an integer.

NB: Dashes (-) and spaces in sample names are automatically converted to underscores (_) to avoid downstream issues in the pipeline.

Nanopore input format

For Nanopore data the pipeline only supports amplicon-based analysis obtained from primer sets created and maintained by the ARTIC Network. The artic minion tool from the ARTIC field bioinformatics pipeline is used to align reads, call variants and to generate the consensus sequence.

Nanopolish

The default variant caller used by artic minion is Nanopolish and this requires that you provide *.fastq, *.fast5 and sequencing_summary.txt files as input to the pipeline. These files can typically be obtained after demultiplexing and basecalling the sequencing data using Guppy (see ARTIC SOP docs). This pipeline requires that the files are organised in the format outlined below and gzip compressed files are also accepted:

.
└── fastq_pass
    └── barcode01
        ├── FAP51364_pass_barcode01_97ca62ca_0.fastq
        ├── FAP51364_pass_barcode01_97ca62ca_1.fastq
        ├── FAP51364_pass_barcode01_97ca62ca_2.fastq
        ├── FAP51364_pass_barcode01_97ca62ca_3.fastq
        ├── FAP51364_pass_barcode01_97ca62ca_4.fastq
        ├── FAP51364_pass_barcode01_97ca62ca_5.fastq
    <TRUNCATED>

.
└── fast5_pass
    ├── barcode01
        ├── FAP51364_pass_barcode01_97ca62ca_0.fast5
        ├── FAP51364_pass_barcode01_97ca62ca_1.fast5
        ├── FAP51364_pass_barcode01_97ca62ca_2.fast5
        ├── FAP51364_pass_barcode01_97ca62ca_3.fast5
        ├── FAP51364_pass_barcode01_97ca62ca_4.fast5
        ├── FAP51364_pass_barcode01_97ca62ca_5.fast5
    <TRUNCATED>

The command to run the pipeline would then be:

nextflow run nf-core/viralrecon \
    --input samplesheet.csv \
    --outdir <OUTDIR> \
    --platform nanopore \
    --genome 'MN908947.3' \
    --primer_set_version 3 \
    --fastq_dir fastq_pass/ \
    --fast5_dir fast5_pass/ \
    --sequencing_summary sequencing_summary.txt \
    -profile <docker/singularity/podman/conda/institute>

Medaka

You also have the option of using Medaka as an alternative variant caller to Nanopolish via the --artic_minion_caller medaka parameter. Medaka is faster than Nanopolish, performs mostly the same and can be run directly from fastq input files as opposed to requiring the fastq, fast5 and sequencing_summary.txt files required to run Nanopolish. You must provide the appropriate Medaka model via the --artic_minion_medaka_model parameter if using --artic_minion_caller medaka. The fastq files have to be organised in the same way as for Nanopolish as outlined in the section above.

The command to run the pipeline would then be:

nextflow run nf-core/viralrecon \
    --input samplesheet.csv \
    --outdir <OUTDIR> \
    --platform nanopore \
    --genome 'MN908947.3' \
    --primer_set_version 3 \
    --fastq_dir fastq_pass/ \
    --artic_minion_caller medaka \
    --artic_minion_medaka_model r941_min_high_g360 \
    -profile <docker/singularity/podman/conda/institute>

Illumina primer sets

The Illumina processing mode of the pipeline has been tested on numerous different primer sets. Where possible we are trying to collate links and settings for standard primer sets to make it easier to run the pipeline with standard parameter keys. If you are able to get permissions from the vendor/supplier to share the primer information then we would be more than happy to support it within the pipeline.

For SARS-CoV-2 data we recommend using the “MN908947.3” genome because it is supported out-of-the-box by the most commonly used primer sets available from the ARTIC Network. For ease of use, we are also maintaining a version of the “MN908947.3” genome along with the appropriate links to the ARTIC primer sets in the genomes config file used by the pipeline. The genomes config file can be updated independently from the main pipeline code to make it possible to dynamically extend this file for other viral genomes/primer sets on request.

For further information or help, don’t hesitate to get in touch on the Slack #viralrecon channel (you can join with this invite).

ARTIC primer sets

An example command using v3 ARTIC primers with “MN908947.3”:

nextflow run nf-core/viralrecon \
    --input samplesheet.csv \
    --outdir <OUTDIR> \
    --platform illumina \
    --protocol amplicon \
    --genome 'MN908947.3' \
    --primer_set artic \
    --primer_set_version 3 \
    --skip_assembly \
    -profile <docker/singularity/podman/conda/institute>

SWIFT primer sets

The SWIFT amplicon panel is another commonly used method used to prep and sequence SARS-CoV-2 samples. We haven’t been able to obtain explicit permission to host standard SWIFT primer sets but you can obtain a masterfile which is freely available from their website that contains the primer sequences as well as genomic co-ordinates. You just need to convert this file to BED6 format and provide it to the pipeline with --primer_bed swift_primers.bed. Be sure to check the values provided to --primer_left_suffix and --primer_right_suffix match the primer names defined in the BED file as highlighted in this issue. For an explanation behind the usage of the --ivar_trim_offset 5 for SWIFT primer sets see this issue.

An example command using SWIFT primers with “MN908947.3”:

nextflow run nf-core/viralrecon \
    --input samplesheet.csv \
    --outdir <OUTDIR> \
    --platform illumina \
    --protocol amplicon \
    --genome 'MN908947.3' \
    --primer_bed swift_primers.bed \
    --primer_left_suffix '_F' \
    --primer_right_suffix '_R' \
    --ivar_trim_offset 5 \
    --skip_assembly \
    -profile <docker/singularity/podman/conda/institute>

Running the pipeline

The typical command for running the pipeline is as follows:

nextflow run nf-core/viralrecon --input samplesheet.csv --outdir <OUTDIR> --genome 'MN908947.3' -profile docker

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:

work                # Directory containing the nextflow working files
<OUTDIR>            # Finished results in specified location (defined with --outdir)
.nextflow_log       # Log file from Nextflow
# Other nextflow hidden files, eg. history of pipeline runs and old logs.

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:

nextflow pull nf-core/viralrecon

Reproducibility

It is 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/viralrecon releases page and find the latest pipeline version - numeric only (eg. 1.3.1). Then specify this when running the pipeline with -r (one hyphen) - eg. -r 1.3.1. Of course, you can switch to another version by changing the number after the -r flag.

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. For example, at the bottom of the MultiQC reports.

Core Nextflow arguments

NB: These options are part of Nextflow and use a single hyphen (pipeline parameters use a double-hyphen).

`-profile`

Use this parameter to choose a configuration profile. Profiles can give configuration presets for different compute environments.

Several generic profiles are bundled with the pipeline which instruct the pipeline to use software packaged using different methods (Docker, Singularity, Podman, Shifter, Charliecloud, Conda) - see below.

We highly recommend the use of Docker or Singularity containers for full pipeline reproducibility, however when this is not possible, Conda is also supported.

The pipeline also dynamically loads configurations from https://github.com/nf-core/configs when it runs, making multiple config profiles for various institutional clusters available at run time. For more information and to see if your system is available in these configs please see the nf-core/configs documentation.

Note that multiple profiles can be loaded, for example: -profile test,docker - the order of arguments is important! They are loaded in sequence, so later profiles can overwrite earlier profiles.

If -profile is not specified, the pipeline will run locally and expect all software to be installed and available on the PATH. This is not recommended, since it can lead to different results on different machines dependent on the computer enviroment.

test
- A profile with a complete configuration for automated testing
- Includes links to test data so needs no other parameters
docker
- A generic configuration profile to be used with Docker
singularity
- A generic configuration profile to be used with Singularity
podman
- A generic configuration profile to be used with Podman
shifter
- A generic configuration profile to be used with Shifter
charliecloud
- A generic configuration profile to be used with Charliecloud
conda
- A generic configuration profile to be used with Conda. Please only use Conda as a last resort i.e. when it’s not possible to run the pipeline with Docker, Singularity, Podman, Shifter or Charliecloud.

`-resume`

Specify this when restarting a pipeline. Nextflow will use cached results from any pipeline steps where the inputs are the same, continuing from where it got to previously. For input to be considered the same, not only the names must be identical but the files’ contents as well. For more info about this parameter, see this blog post.

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.

`-c`

Specify the path to a specific config file (this is a core Nextflow command). See the nf-core website documentation for more information.

Custom configuration

Resource requests

Whilst the default requirements set within the pipeline will hopefully work for most people and with most input data, you may find that you want to customise the compute resources that the pipeline requests. 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 any of the error codes specified here it will automatically be resubmitted with higher requests (2 x original, then 3 x original). If it still fails after the third attempt then the pipeline execution is stopped.

For example, if the nf-core/rnaseq pipeline is failing after multiple re-submissions of the STAR_ALIGN process due to an exit code of 137 this would indicate that there is an out of memory issue:

[62/149eb0] NOTE: Process `NFCORE_RNASEQ:RNASEQ:ALIGN_STAR:STAR_ALIGN (WT_REP1)` terminated with an error exit status (137) -- Execution is retried (1)
Error executing process > 'NFCORE_RNASEQ:RNASEQ:ALIGN_STAR:STAR_ALIGN (WT_REP1)'
 
Caused by:
    Process `NFCORE_RNASEQ:RNASEQ:ALIGN_STAR:STAR_ALIGN (WT_REP1)` terminated with an error exit status (137)
 
Command executed:
    STAR \
        --genomeDir star \
        --readFilesIn WT_REP1_trimmed.fq.gz  \
        --runThreadN 2 \
        --outFileNamePrefix WT_REP1. \
        <TRUNCATED>
 
Command exit status:
    137
 
Command output:
    (empty)
 
Command error:
    .command.sh: line 9:  30 Killed    STAR --genomeDir star --readFilesIn WT_REP1_trimmed.fq.gz --runThreadN 2 --outFileNamePrefix WT_REP1. <TRUNCATED>
Work dir:
    /home/pipelinetest/work/9d/172ca5881234073e8d76f2a19c88fb
 
Tip: you can replicate the issue by changing to the process work dir and entering the command `bash .command.run`

For beginners

A first step to bypass this error, you could try to increase the amount of CPUs, memory, and time for the whole pipeline. Therefor you can try to increase the resource for the parameters --max_cpus, --max_memory, and --max_time. Based on the error above, you have to increase the amount of memory. Therefore you can go to the parameter documentation of rnaseq and scroll down to the show hidden parameter button to get the default value for --max_memory. In this case 128GB, you than can try to run your pipeline again with --max_memory 200GB -resume to skip all process, that were already calculated. If you can not increase the resource of the complete pipeline, you can try to adapt the resource for a single process as mentioned below.

Advanced option on process level

To bypass this error you would need to find exactly which resources are set by the STAR_ALIGN process. The quickest way is to search for process STAR_ALIGN in the nf-core/rnaseq Github repo. We have standardised the structure of Nextflow DSL2 pipelines such that all module files will be present in the modules/ directory and so, based on the search results, the file we want is modules/nf-core/star/align/main.nf. If you click on the link to that file you will notice that there is a label directive at the top of the module that is set to label process_high. The Nextflow label directive allows us to organise workflow processes in separate groups which can be referenced in a configuration file to select and configure subset of processes having similar computing requirements. The default values for the process_high label are set in the pipeline’s base.config which in this case is defined as 72GB. Providing you haven’t set any other standard nf-core parameters to cap the maximum resources used by the pipeline then we can try and bypass the STAR_ALIGN process failure by creating a custom config file that sets at least 72GB of memory, in this case increased to 100GB. The custom config below can then be provided to the pipeline via the -c parameter as highlighted in previous sections.

process {
    withName: 'NFCORE_RNASEQ:RNASEQ:ALIGN_STAR:STAR_ALIGN' {
        memory = 100.GB
    }
}

NB: We specify the full process name i.e. NFCORE_RNASEQ:RNASEQ:ALIGN_STAR:STAR_ALIGN in the config file because this takes priority over the short name (STAR_ALIGN) and allows existing configuration using the full process name to be correctly overridden.

If you get a warning suggesting that the process selector isn’t recognised check that the process name has been specified correctly.

Updating containers (advanced users)

The Nextflow DSL2 implementation of this pipeline uses one container per process which makes it much easier to maintain and update software dependencies. If for some reason you need to use a different version of a particular tool with the pipeline then you just need to identify the process name and override the Nextflow container definition for that process using the withName declaration. For example, in the nf-core/viralrecon pipeline a tool called Pangolin has been used during the COVID-19 pandemic to assign lineages to SARS-CoV-2 genome sequenced samples. Given that the lineage assignments change quite frequently it doesn’t make sense to re-release the nf-core/viralrecon everytime a new version of Pangolin has been released. However, you can override the default container used by the pipeline by creating a custom config file and passing it as a command-line argument via -c custom.config.

Pangolin

For example, in the nf-core/viralrecon pipeline a tool called Pangolin has been used during the COVID-19 pandemic to assign lineages to SARS-CoV-2 genome sequenced samples. Given that the lineage assignments change quite frequently it doesn’t make sense to re-release the nf-core/viralrecon everytime a new version of Pangolin has been released. However, you can override the default container used by the pipeline by creating a custom config file and passing it as a command-line argument via -c custom.config.

Check the default version used by the pipeline in the module file for Pangolin
Find the latest version of the Biocontainer available on Quay.io

Create the custom config accordingly:

For Docker:

process {
    withName: PANGOLIN {
        container = 'quay.io/biocontainers/pangolin:3.1.17--pyhdfd78af_1'
    }
}

For Singularity:

process {
    withName: PANGOLIN {
        container = 'https://depot.galaxyproject.org/singularity/pangolin:3.1.17--pyhdfd78af_1'
    }
}

For Conda:

process {
    withName: PANGOLIN {
        conda = 'bioconda::pangolin=3.1.17'
    }
}

Nextclade

You can use a similar approach to update the version of Nextclade used by the pipeline:

Check the default version used by the pipeline in the module file for Nextclade
Find the latest version of the Biocontainer available on Quay.io

Create the custom config accordingly:

For Docker:

process {
    withName: 'NEXTCLADE_DATASETGET|NEXTCLADE_RUN' {
        container = 'quay.io/biocontainers/nextclade:1.10.1--h9ee0642_0'
    }
}

For Singularity:

process {
    withName: 'NEXTCLADE_DATASETGET|NEXTCLADE_RUN' {
        container = 'https://depot.galaxyproject.org/singularity/nextclade:1.10.1--h9ee0642_0'
    }
}

For Conda:

process {
    withName: 'NEXTCLADE_DATASETGET|NEXTCLADE_RUN' {
        conda = 'bioconda::nextclade=1.10.1'
    }
}

Nextclade datasets

A nextclade dataset feature was introduced in Nextclade CLI v1.3.0 that fetches input genome files such as reference sequences and trees from a central dataset repository. We have uploaded Nextclade dataset v2022-06-14 to nf-core/test-datasets, and for reproducibility, this will be used by default if you specify --genome 'MN908947.3' when running the pipeline. However, there are a number of ways you can use a more recent version of the dataset:

Supply your own by setting: --nextclade_dataset <PATH_TO_DATASET>
Let the pipeline create and use the latest version by setting: --nextclade_dataset false --nextclade_dataset_tag false
Let the pipeline create and use a specific, tagged version by setting: --nextclade_dataset false --nextclade_dataset_tag <DATASET_TAG>

The Nextclade dataset releases can be found on their Github page. Use the tag specified for each release e.g 2022-01-18T12:00:00Z in the example below:

Nextclade tag example

If the --save_reference parameter is provided then the Nextclade dataset generated by the pipeline will also be saved in the results/genome/ directory.

NB: If you wish to periodically update individual tool-specific results (e.g. Pangolin) generated by the pipeline then you must ensure to keep the work/ directory otherwise the -resume ability of the pipeline will be compromised and it will restart from scratch.

nf-core/configs

In most cases, you will only need to create a custom config as a one-off but if you and others within your organisation are likely to be running nf-core pipelines regularly and need to use the same settings 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. 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.

See the main Nextflow documentation for more information about creating your own configuration files.

If you have any questions or issues please send us a message on Slack on the #configs channel.

Azure Resource Requests

To be used with the azurebatch profile by specifying the -profile azurebatch. We recommend providing a compute params.vm_type of Standard_D16_v3 VMs by default but these options can be changed if required.

Note that the choice of VM size depends on your quota and the overall workload during the analysis. For a thorough list, please refer the Azure Sizes for virtual machines in Azure.

Running in the background

Nextflow handles job submissions and supervises the running jobs. The Nextflow process must run until the pipeline is finished.

The Nextflow -bg flag launches Nextflow in the background, detached from your terminal so that the workflow does not stop if you log out of your session. The logs are saved to a file.

Alternatively, you can use screen / tmux or similar tool to create a detached session which you can log back into at a later time. Some HPC setups also allow you to run nextflow within a cluster job submitted your job scheduler (from where it submits more jobs).

Nextflow memory requirements

In some cases, the Nextflow Java virtual machines can start to request a large amount of memory. We recommend adding the following line to your environment to limit this (typically in ~/.bashrc or ~./bash_profile):

NXF_OPTS='-Xms1g -Xmx4g'

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nf-core/viralrecon Edit