nf-core/rnavar

Path to comma-separated file containing information about the samples in the experiment.

The output directory where the results will be saved. You have to use absolute paths to storage on Cloud infrastructure.

Email address for completion summary.

MultiQC report title. Printed as page header, used for filename if not otherwise specified.

Save FastQ files after merging re-sequenced libraries in the results directory.

Name of iGenomes reference.

Path to FASTA genome file.

Path to FASTA dictionary file.

Path to FASTA reference index.

Path to GTF annotation file.

Path to GFF3 annotation file.

Path to BED file containing exon intervals. This will be created from the GTF file if not specified.

Read length

If generated by the pipeline, save the STAR index in the results directory.

Path to known indels VCF file(s)

Path to known indels index file(s)

Path to dbSNP VCF file

Path to dbSNP VCF index file

snpEff DB version.

VEP genome.

VEP species.

VEP cache version.

Type of feature to parse from annotation file

Download annotation cache.

Specify whether to remove duplicates from the BAM during Picard MarkDuplicates step.

Specifies the alignment algorithm to use.

Path to STAR index folder or compressed file (tar.gz)

Enable STAR 2-pass mapping mode.

Do not use GTF file during STAR index building step

Option to limit RAM when sorting BAM file. Value to be specified in bytes. If 0, will be set to the genome index size.

Specifies the number of genome bins for coordinate-sorting

Specifies the maximum number of collapsed junctions

Specifies the maximum intron size

Sequencing center information to be added to read group of BAM files.

Specify the sequencing platform used

Where possible, save unaligned reads from aligner to the results directory.

Save the intermediate BAM files from the alignment step.

Create a CSI index for BAM files instead of the traditional BAI index. This will be required for genomes with larger chromosome sizes.

Specify whether to remove UMIs from the reads with UMI-tools extract.

UMI pattern to use. Can be either ‘string’ (default) or ‘regex’.

The UMI barcode pattern to use e.g. ‘NNNNNN’ indicates that the first 6 nucleotides of the read are from the UMI.

The UMI barcode pattern to use if the UMI is located in read 2.

The character that separates the UMI in the read name. Most likely a colon if you skipped the extraction with UMI-tools and used other software.

The minimum phred-scaled confidence threshold at which variants should be called.

Enable generation of GVCFs by sample additionnaly to the VCFs.

Path to VEP cache.

Path to snpEff cache.

Enable the use of the VEP dbNSFP plugin.

Path to dbNSFP processed file.

Path to dbNSFP tabix indexed file.

Consequence to annotate with

Fields to annotate with

Enable the use of the VEP LOFTEE plugin.

Enable the use of the VEP SpliceAI plugin.

Path to spliceai raw scores snv file.

Path to spliceai raw scores snv tabix indexed file.

Path to spliceai raw scores indel file.

Path to spliceai raw scores indel tabix indexed file.

Enable the use of the VEP SpliceRegion plugin.

Add an extra custom argument to VEP.

Skip the process of base recalibration steps i.e., GATK BaseRecalibrator and GATK ApplyBQSR.

Skip the process of preparing interval lists for the GATK variant calling step

Skip variant filtering of GATK

Skip variant annotation

Skip MultiQC reports

Skip the check of the exon bed

Number of times the gene interval list to be split in order to run GATK haplotype caller in parallel

Do not use gene interval file during variant calling

The window size (in bases) in which to evaluate clustered SNPs.

The number of SNPs which make up a cluster. Must be at least 2.

Value to be used for the FisherStrand (FS) filter

Value to be used for the QualByDepth (QD) filter

Custom MultiQC yaml file containing HTML including a methods description.