5 Base DNA Somatic Tumor-Normal Solid WGS

A DRAGEN recipe, like this one, is a predefined set of analysis parameters and workflow settings tailored to a specific type of genomic analysis. For clarity, some default parameters are explicitly included and annotated with comments. This recipe includes the recommended commands for solid samples. These settings support fresh frozen samples, as well as some optional settings for FFPE samples.

  
/opt/dragen/$VERSION/bin/dragen         #DRAGEN install path 
--ref-dir $REF_DIR                      #path to DRAGEN linear hashtable 
--output-directory $OUTPUT 
--intermediate-results-dir $PATH        #e.g. SSD /staging 
--output-file-prefix $PREFIX 
# Inputs 
--tumor-fastq-list $PATH                #see 'Input Options' for FQ, BAM or CRAM 
--tumor-fastq-list-sample-id $STRING 
--fastq-list $PATH                      #see 'Input Options' for FQ, BAM or CRAM 
--fastq-list-sample-id $STRING 
# Mapper 
--enable-map-align true                 #optional with BAM/CRAM input 
--enable-map-align-output true          #optionally save the output BAM 
--enable-sort true                      #default=true 
--enable-duplicate-marking true         #default=true 
# 5-Base 
--methylation-conversion illumina 
--methylation-generate-cytosine-report true 
--methylation-compress-cx-report true 
# Small variant caller 
--enable-variant-caller true 
--vc-systematic-noise $PATH             #Recommended 
--vc-excluded-regions-bed $BED          #FFPE: optionally mask ALUs 
# CNV 
--enable-cnv true 
--cnv-use-somatic-vc-baf true 
--cnv-enable-self-normalization true 
# Annotation 
--variant-annotation-data PATH 
--enable-variant-annotation true

Notes and additional options

Hashtable

For DRAGEN somatic runs it is recommended to use the linear hashtable.

See: Product Files

Input options

DRAGEN input sources include: fastq list, fastq, bam, or cram. For BCL input, first create FASTQs using BCL conversion.

FQ list Input

--tumor-fastq-list $PATH 
--tumor-fastq-list-sample-id $STRING 
--fastq-list $PATH 
--fastq-list-sample-id $STRING

FQ Input

--tumor-fastq1 $PATH 
--tumor-fastq2 $PATH 
--RGSM-tumor $STRING 
--RGID-tumor $STRING 
--fastq-file1 $PATH 
--fastq-file2 $PATH 
--RGSM $STRING 
--RGID $STRING

BAM Input

--tumor-bam-input $PATH 
--bam-input $PATH

CRAM Input

--tumor-cram-input $PATH 
--cram-input $PATH

Mapping and Aligning

Option

Description

--enable-map-align true

In the TN pipeline this must be set to false for BAM/CRAM input.

--enable-map-align-output true

Optionally save the output BAM (default=false).

--Aligner.clip-pe-overhang 2

Clean up any unwanted UMI indexes. Only use when reads contain UMIs, but UMI collapsing was not run.

Duplicate Marking

Option

Description

--enable-duplicate-marking true

By default, DRAGEN marks duplicate reads and exclude them from variant calling.

Fractional (Raw Reads) Downsampling

DRAGEN can subsample a random, fractional percentage of reads from an input file using the fractional downsampler. You can use downsampling to subsample data sets in order to simulate different amounts of sequencing. DRAGEN randomly subsamples reads from primary analysis without any modification (e.g. no trimming, no filtering, etc.).

Downsampling may be useful to reduce runtime on very deep samples. For Tumor-Normal analyses it is also recommended to use a normal sample with coverage that is less than the tumor sample. If the matched normal has deeper coverage than the tumor sample, then the fractional samples may be used to reduce coverage on the normal sample.

Option

Description

--enable-fractional-down-sampler

Set to true to enable fractional downsampling. The default value is false.

--down-sampler-normal-subsample

Specify the fraction of reads to keep as a subsample of normal input data. The default value is 1.0 (100%).

--down-sampler-tumor-subsample

Specify the fraction of reads to keep as a subsample of tumor input data. The default value is 1.0 (100%).

--down-sampler-random-seed

Specify the random seed for different runs of the same input data. The default value is 42.

5-Base Methylation

Option

Description

--methylation-conversion STRING

Library conversion for methylation analysis. Options: none, c_t, mc_t, illumina (default=none).

--methylation-protocol STRING

Library protocol for methylation analysis. Options: none, directional, non-directional, directional-complement, pbat. The default value for methylation-conversion=illumina is directional, otherwise it is none.

--methylation-mapq-threshold INT

Only reads with MAPQ greater or equal than the threshold will be included in methyl-seq analysis (default=0).

--methylation-generate-mbias-report true

Whether to generate a per-sequencer-cycle methylation bias report (default=true).

--mbias-report-include-overlaps

Calculate methylation stats for overlapping bases between mates (default=false).

--methylation-generate-cytosine-report true

Whether to generate a genome-wide cytosine methylation CX_report file (default=false).

--methylation-compress-cx-report true

Set to true to enable compression of the CX_report (default=true).

--methylation-keep-ref-cytosine true

Set to true to keep all reference cytosines in the CX_report file, even if they don't appear in the input reads (default=false).

--enable-cpg-methylated-mapping true

Enable methylated mapping with base conversions restricted to CpG context (default=true). When false, runs DRAGEN Methylation 3-base map/align instead.

--methylation-report-to-vcf

Specify methylation type (none, cg, or c) which is reported in VCF files (default=c).

--methylation-report-to-gvcf

Specify methylation type (none, cg, or c) which is reported in gVCF files (default=cg).

For more information see: 5-Base Pipeline.

SNV

Option

Description

--vc-target-bed

Limit variant calling to region of interest.

--vc-combine-phased-variants-distance INT

Maximum distance in base pairs (BP) over which phased variants will be combined. Set to 0 to disable. Valid range is [0; 15] BP (Default=2)

--vc-systematic-noise $PATH

Systematic noise file. This filter is recommended for removing systematic noise observed in normal samples (i.e. systematic alignment errors, sequencing errors, etc.).

--vc-somatic-hotspots $PATH

DRAGEN has a default set of hotspot variants (positions and alleles) where it will assign an increased prior probability. Use this option to override with a custom hotspots file.

--vc-enable-liquid-tumor-mode true

Tumor-in-normal contamination. Only use if there is some tumor leakage in the normal control.

--vc-override-tumor-pcr-params-with-normal false

Mixed sample preparation. Only use if the tumor and normal samples exhibit different PCR (indel) noise patterns, e.g., due to using different sample preparation.

--vc-sq-filter-threshold $NUM

Threshold for sensitivity-specificity tradeoff using SQ score. The pipeline specific default threshold is 17.5. Raise this value to improve specificity at the cost of sensitivity, or lower it to improve sensitivity at the cost of specificity.

--vc-systematic-noise-filter-threshold $INT

Threshold for sensitivity-specificty tradeoff using AQ score for non-hotspot variants. This is only used when supplying a systematic noise file. Pipeline specific default value = 10. Raise this value to improve specificity at the cost of sensitivity, or lower it to improve sensitivity at the cost of specificity.

--vc-systematic-noise-filter-threshold-in-hotspot $INT

Threshold for sensitivity-specificty tradeoff using AQ score for hotspot variants. This is only used when supplying a systematic noise file. Pipeline specific default value = 10. Raise this value to improve specificity at the cost of sensitivity, or lower it to improve sensitivity at the cost of specificity.

--vc-excluded-regions-bed $BED

Hard filter variants that overlap with this region. ALU regions comprise approximately 11% of the genome, and are often exceptionally noisy regions in FFPE samples. Optionally filter out ALU regions using the DRAGEN excluded regions filter. ALU bed files can be downloaded as part of the Bed File Collection: Bed File Collection

For more detail on the small variant caller in somatic mode please refer to Somatic Mode

CNV

Option

Description

--cnv-enable-gcbias-correction true

Enable or disable GC bias correction when generating target counts.

--cnv-segmentation-mode $SEG_MODE

Option to override the default segmentation algorithm. Defaults include slm for germline WGS, aslm for somatic WGS, and hslm for targeted analysis.

--cnv-normal-cnv-vcf $CNV_NORMAL_VCF

Specify germline CNVs from the matched normal sample. Germline-aware Mode.

For more information, see CNV Calling.

Annotation

For instructions on how to download the Nirvana annotation database, please refer to Nirvana

Resource Files

DRAGEN requires resource files for components such as SNV, SV, and CNV. The following notes provide references for downloading these files or generating them for custom workflows or assays.

SNV Systematic Noise

Systematic noise files are considered essential in Tumor-Only workflows. It is also recommended for Tumor-Normals workflows.

DRAGEN has pre-build systematic noise files for WES/WGS. These files should also be used in 5-Base workflows. The 5-Base workflows have not been tested with custom noise files.

Prebuild

Prebuilt systematic noise BED files (WES and WGS) can be downloaded here: Product Files.

Prebuilt WES/WGS noise files

Description

WGS_hg38_v2.0.0_systematic_noise.snv.bed.gz

For WGS FF

FFPE_WGS_hg38_v2.0.0_systematic_noise.snv.bed.gz

For WGS FFPE (only hg38)

WES_hg38_v2.0.0_systematic_noise.snv.bed.gz

For WES FF and FFPE

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