millironx/taxprofiler
1
0
Fork 0
mirror of https://github.com/MillironX/taxprofiler.git synced 2024-09-21 04:22:04 +00:00
Code Issues Releases Packages Activity

Add samtools stats for short-reads

Browse source
This commit is contained in:
Sofia Stamouli 2022-10-28 14:24:33 +02:00
parent bf89525bc2
commit 5b99d9024a
8 changed files with 236 additions and 0 deletions
Show stats Download patch file Download diff file Expand all files Collapse all files

1
assets/multiqc_config.yml
View file

@ -21,6 +21,7 @@ run_modules:
- adapterRemoval
- fastp
- bowtie2
- samtools
- kraken
- malt
- custom_content

12
conf/modules.config
View file

@ -233,6 +233,18 @@ process {
]
}
withName: SAMTOOLS_STATS {
ext.prefix = { "${meta.id}_${meta.run_accession}" }
publishDir = [
path: { "${params.outdir}/samtools/stats" },
mode: params.publish_dir_mode,
enabled: params.save_hostremoval_unmapped,
pattern: '*stats'
]
}
withName: BBMAP_BBDUK {
ext.args = [
"entropy=${params.shortread_complexityfilter_entropy}",

8
modules.json
View file

@ -153,6 +153,14 @@
"branch": "master",
"git_sha": "5e34754d42cd2d5d248ca8673c0a53cdf5624905"
},
"samtools/index": {
"branch": "master",
"git_sha": "5e34754d42cd2d5d248ca8673c0a53cdf5624905"
},
"samtools/stats": {
"branch": "master",
"git_sha": "5e34754d42cd2d5d248ca8673c0a53cdf5624905"
},
"samtools/view": {
"branch": "master",
"git_sha": "5e34754d42cd2d5d248ca8673c0a53cdf5624905"

48
modules/nf-core/samtools/index/main.nf generated Normal file
View file

@ -0,0 +1,48 @@
process SAMTOOLS_INDEX {
tag "$meta.id"
label 'process_low'
conda (params.enable_conda ? "bioconda::samtools=1.15.1" : null)
container "${ workflow.containerEngine == 'singularity' && !task.ext.singularity_pull_docker_container ?
'https://depot.galaxyproject.org/singularity/samtools:1.15.1--h1170115_0' :
'quay.io/biocontainers/samtools:1.15.1--h1170115_0' }"
input:
tuple val(meta), path(input)
output:
tuple val(meta), path("*.bai") , optional:true, emit: bai
tuple val(meta), path("*.csi") , optional:true, emit: csi
tuple val(meta), path("*.crai"), optional:true, emit: crai
path "versions.yml" , emit: versions
when:
task.ext.when == null || task.ext.when
script:
def args = task.ext.args ?: ''
"""
samtools \\
index \\
-@ ${task.cpus-1} \\
$args \\
$input
cat <<-END_VERSIONS > versions.yml
"${task.process}":
samtools: \$(echo \$(samtools --version 2>&1) | sed 's/^.*samtools //; s/Using.*\$//')
END_VERSIONS
"""
stub:
"""
touch ${input}.bai
touch ${input}.crai
touch ${input}.csi
cat <<-END_VERSIONS > versions.yml
"${task.process}":
samtools: \$(echo \$(samtools --version 2>&1) | sed 's/^.*samtools //; s/Using.*\$//')
END_VERSIONS
"""
}

53
modules/nf-core/samtools/index/meta.yml generated Normal file
View file

@ -0,0 +1,53 @@
name: samtools_index
description: Index SAM/BAM/CRAM file
keywords:
- index
- bam
- sam
- cram
tools:
- samtools:
description: |
SAMtools is a set of utilities for interacting with and post-processing
short DNA sequence read alignments in the SAM, BAM and CRAM formats, written by Heng Li.
These files are generated as output by short read aligners like BWA.
homepage: http://www.htslib.org/
documentation: hhttp://www.htslib.org/doc/samtools.html
doi: 10.1093/bioinformatics/btp352
licence: ["MIT"]
input:
- meta:
type: map
description: |
Groovy Map containing sample information
e.g. [ id:'test', single_end:false ]
- bam:
type: file
description: BAM/CRAM/SAM file
pattern: "*.{bam,cram,sam}"
output:
- meta:
type: map
description: |
Groovy Map containing sample information
e.g. [ id:'test', single_end:false ]
- bai:
type: file
description: BAM/CRAM/SAM index file
pattern: "*.{bai,crai,sai}"
- crai:
type: file
description: BAM/CRAM/SAM index file
pattern: "*.{bai,crai,sai}"
- csi:
type: file
description: CSI index file
pattern: "*.{csi}"
- versions:
type: file
description: File containing software versions
pattern: "versions.yml"
authors:
- "@drpatelh"
- "@ewels"
- "@maxulysse"

49
modules/nf-core/samtools/stats/main.nf generated Normal file
View file

@ -0,0 +1,49 @@
process SAMTOOLS_STATS {
tag "$meta.id"
label 'process_single'
conda (params.enable_conda ? "bioconda::samtools=1.15.1" : null)
container "${ workflow.containerEngine == 'singularity' && !task.ext.singularity_pull_docker_container ?
'https://depot.galaxyproject.org/singularity/samtools:1.15.1--h1170115_0' :
'quay.io/biocontainers/samtools:1.15.1--h1170115_0' }"
input:
tuple val(meta), path(input), path(input_index)
path fasta
output:
tuple val(meta), path("*.stats"), emit: stats
path "versions.yml" , emit: versions
when:
task.ext.when == null || task.ext.when
script:
def args = task.ext.args ?: ''
def prefix = task.ext.prefix ?: "${meta.id}"
def reference = fasta ? "--reference ${fasta}" : ""
"""
samtools \\
stats \\
--threads ${task.cpus} \\
${reference} \\
${input} \\
> ${prefix}.stats
cat <<-END_VERSIONS > versions.yml
"${task.process}":
samtools: \$(echo \$(samtools --version 2>&1) | sed 's/^.*samtools //; s/Using.*\$//')
END_VERSIONS
"""
stub:
def prefix = task.ext.prefix ?: "${meta.id}"
"""
touch ${prefix}.stats
cat <<-END_VERSIONS > versions.yml
"${task.process}":
samtools: \$(echo \$(samtools --version 2>&1) | sed 's/^.*samtools //; s/Using.*\$//')
END_VERSIONS
"""
}

53
modules/nf-core/samtools/stats/meta.yml generated Normal file
View file

@ -0,0 +1,53 @@
name: samtools_stats
description: Produces comprehensive statistics from SAM/BAM/CRAM file
keywords:
- statistics
- counts
- bam
- sam
- cram
tools:
- samtools:
description: |
SAMtools is a set of utilities for interacting with and post-processing
short DNA sequence read alignments in the SAM, BAM and CRAM formats, written by Heng Li.
These files are generated as output by short read aligners like BWA.
homepage: http://www.htslib.org/
documentation: hhttp://www.htslib.org/doc/samtools.html
doi: 10.1093/bioinformatics/btp352
licence: ["MIT"]
input:
- meta:
type: map
description: |
Groovy Map containing sample information
e.g. [ id:'test', single_end:false ]
- input:
type: file
description: BAM/CRAM file from alignment
pattern: "*.{bam,cram}"
- input_index:
type: file
description: BAI/CRAI file from alignment
pattern: "*.{bai,crai}"
- fasta:
type: optional file
description: Reference file the CRAM was created with
pattern: "*.{fasta,fa}"
output:
- meta:
type: map
description: |
Groovy Map containing sample information
e.g. [ id:'test', single_end:false ]
- stats:
type: file
description: File containing samtools stats output
pattern: "*.{stats}"
- versions:
type: file
description: File containing software versions
pattern: "versions.yml"
authors:
- "@drpatelh"
- "@FriederikeHanssen"

12
subworkflows/local/shortread_hostremoval.nf
View file

@ -4,6 +4,8 @@
include { BOWTIE2_BUILD } from '../../modules/nf-core/bowtie2/build/main'
include { BOWTIE2_ALIGN } from '../../modules/nf-core/bowtie2/align/main'
include { SAMTOOLS_INDEX } from '../../modules/nf-core/samtools/index/main'
include { SAMTOOLS_STATS } from '../../modules/nf-core/samtools/stats/main'
workflow SHORTREAD_HOSTREMOVAL {
take:
@ -26,7 +28,17 @@ workflow SHORTREAD_HOSTREMOVAL {
ch_versions = ch_versions.mix( BOWTIE2_ALIGN.out.versions.first() )
ch_multiqc_files = ch_multiqc_files.mix( BOWTIE2_ALIGN.out.log )
SAMTOOLS_INDEX ( BOWTIE2_ALIGN.out.bam )
bam_bai = BOWTIE2_ALIGN.out.bam
.join(SAMTOOLS_INDEX.out.bai, remainder: true)
SAMTOOLS_STATS ( bam_bai, reference )
ch_versions = ch_versions.mix(SAMTOOLS_STATS.out.versions.first())
ch_multiqc_files = ch_multiqc_files.mix( SAMTOOLS_STATS.out.stats )
emit:
stats = SAMTOOLS_STATS.out.stats
reads = BOWTIE2_ALIGN.out.fastq // channel: [ val(meta), [ reads ] ]
versions = ch_versions // channel: [ versions.yml ]
mqc = ch_multiqc_files