nf-core_modules/modules/samtools/bam2fq/meta.yml

name: samtools_bam2fq
description: |
    The module uses bam2fq method from samtools to
    convert a SAM, BAM or CRAM file to FASTQ format
keywords:
  - bam2fq
  - samtools
  - fastq
tools:
  - samtools:
      description: Tools for dealing with SAM, BAM and CRAM files
      homepage: None
      documentation: http://www.htslib.org/doc/1.1/samtools.html
      tool_dev_url: None
      doi: ""
      licence: ['MIT']

input:
  - meta:
      type: map
      description: |
        Groovy Map containing sample information
        e.g. [ id:'test', single_end:false ]
  - inputbam:
      type: file
      description: BAM/CRAM/SAM file
      pattern: "*.{bam,cram,sam}"
  - split:
      type: boolean
      description: |
        TRUE/FALSE value to indicate if reads should be separated into
        /1, /2 and if present other, or singleton.
        Note: choosing TRUE will generate 4 different files.
        Choosing FALSE will produce a single file, which will be interleaved in case
        the input contains paired reads.

output:
  - meta:
      type: map
      description: |
        Groovy Map containing sample information
        e.g. [ id:'test', single_end:false ]
  - versions:
      type: file
      description: File containing software versions
      pattern: "versions.yml"
  - reads:
      type: file
      description: |
        FASTQ files, which will be either a group of 4 files (read_1, read_2, other and singleton)
        or a single interleaved .fq.gz file if the user chooses not to split the reads.
      pattern: "*.fq.gz"

authors:
  - "@lescai"
Bam2fq (#958) * added template for module * update main * added specific code * wrong variable name in else script * added tests for both split and nosplit * docker test successful - updating yaml * adding echo to version print 2021-10-29 08:46:34 +00:00			`name: samtools_bam2fq`
			`description: \|`
			`The module uses bam2fq method from samtools to`
			`convert a SAM, BAM or CRAM file to FASTQ format`
			`keywords:`
			`- bam2fq`
			`- samtools`
			`- fastq`
			`tools:`
			`- samtools:`
			`description: Tools for dealing with SAM, BAM and CRAM files`
			`homepage: None`
			`documentation: http://www.htslib.org/doc/1.1/samtools.html`
			`tool_dev_url: None`
			`doi: ""`
			`licence: ['MIT']`

			`input:`
			`- meta:`
			`type: map`
			`description: \|`
			`Groovy Map containing sample information`
			`e.g. [ id:'test', single_end:false ]`
			`- inputbam:`
			`type: file`
			`description: BAM/CRAM/SAM file`
			`pattern: "*.{bam,cram,sam}"`
			`- split:`
			`type: boolean`
			`description: \|`
			`TRUE/FALSE value to indicate if reads should be separated into`
			`/1, /2 and if present other, or singleton.`
			`Note: choosing TRUE will generate 4 different files.`
			`Choosing FALSE will produce a single file, which will be interleaved in case`
			`the input contains paired reads.`

			`output:`
			`- meta:`
			`type: map`
			`description: \|`
			`Groovy Map containing sample information`
			`e.g. [ id:'test', single_end:false ]`
			`- versions:`
			`type: file`
			`description: File containing software versions`
			`pattern: "versions.yml"`
			`- reads:`
			`type: file`
			`description: \|`
			`FASTQ files, which will be either a group of 4 files (read_1, read_2, other and singleton)`
			`or a single interleaved .fq.gz file if the user chooses not to split the reads.`
			`pattern: "*.fq.gz"`

			`authors:`
			`- "@lescai"`