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Nextflow Data Processing & Configuration

Owned by Robert Allaway
Last updated: Oct 23, 2023Version comment
3 min read

Our pipeline configuration is still in-development, and the contents of this document are subject to change.

Summary of Processing

https://nf-co.re/sarek/usage v3.0

Datatype

Method

Output

Tried yet?

WES or WGS

DeepVariant

Germline SNV, INDEL

Yes

WES or WGS

Strelka, Mutect2

Somatic SNV, INDEL

Yes

WES or WGS

TBD

Germline and Somatic Structural Variants

No

WES or WGS

TBD

Germline and Somatic CNV

No

WES or WGS

TBD

Tumor MSI

No

SNV, INDEL variants

TBD

Annotated Variants

No

 

https://nf-co.re/rnaseq v3.7

Datatype

Method

Output

Tried yet?

RNA-Seq

STAR with Salmon in alignment-based mode

Gene expression counts

Yes

More information about the workflows is available here: https://sagebionetworks.jira.com/wiki/spaces/WF/pages/2363359776

bam/cram to fastq conversion

  • When fastq files are not available, cram/bam files are converted to fastq using this pipeline: https://github.com/qbic-pipelines/bamtofastq (v1.2.0).

  • If unaligned bam files are available instead of fastq files, we recommend providing u-bam files for direct input to sarek 3.0.

WES and WGS Variant Calling (SNV & INDEL)

Germline SNV + INDEL

This involves transformation of WES fastq or cram files to variant call files in VCF format (.vcf files).

As of Jan 2022, the reference genome used is Homo_sapiens/GATK/GRCh38 (https://github.com/nf-core/sarek/blob/2.7.1/conf/igenomes.config#L38-L58)

The processing steps include the following:

  • Raw fastq files uploaded to Synapse by researcher in a folder with name format experiment_name_rnaseq_fastq_date. No white space should be present in the filenames (all filenames should have _ for whitespaces.

  • All experiment and sample related annotations need to be added on Synapse before processing can start. This is a required step so that a sample sheet can be generated to trigger the processing workflow

  • The sample sheet should contain the following information in a comma-separated file (.csv) with at least 3 columns, and a header row as shown below. (More information here)

sample

subject

status

sex

file_1

file_2

lane

parentId

bed_file

output_parent_Id

Synapse specimenID

Synapse individualID

1 (Tumor = 1, Normal 0)

XX or XY

syn://synId

syn://synId

Lane information

SynapseID of parent folder

Synapse ID of BED file (if WES sata)

Synapse ID of folder where all processed files will be indexed

  • The files are pulled into NextFlow workflow setup and processed using the following versions of software:

nf-core/sarek v2.7.1 Nextflow v21.10.5 BWA 0.7.17 GATK v4.1.7.0 FreeBayes v1.3.2 samtools v1.9 Strelka v2.9.10 Manta v1.6.0 TIDDIT v2.7.1 AlleleCount v4.0.2 ASCAT v2.5.2 Control-FREEC vv11.6 msisensor v0.5 SnpEff v4.3t VEP v99.2 MultiQC v1.8 FastQC v0.11.9 bcftools v1.9 CNVkit v0.9.6 htslib v1.9 QualiMap v2.2.2-dev Trim Galore v0.6.4_dev vcftools v0.1.16 R v4.0.2

 

Commands used for running JHU samples on DeepVariant:

All files and sample sheets are first staged in S3 buckets linked to NFTower. then the following command are used to launch the processing pipeline.

Params:

input: s3://jhu-biobank-nf-project-tower-bucket/jobs/02-sage-sarek-2.7.1-deepvariant/inputs/sample-sheet.tsv outdir: s3://jhu-biobank-nf-project-tower-bucket/jobs/02-sage-sarek-2.7.1-deepvariant/outputs/ genome: GRCh38 igenomes_base: s3://sage-igenomes/igenomes model_type: WES tools: "deepvariant"

Config:

process { errorStrategy = 'retry' maxRetries = 3 withLabel:deepvariant { container = "google/deepvariant:1.1.0" cpus = 24 } }

Pre-run Script:

Profiles:

 

Somatic SNV + INDEL

TBD

 

Annotated Variants

Currently, germline variant calls in VCF format are being processed manually using VEP and vcf2maf

 

RNA Sequencing Data Quantification

Processing RNA-seq files involve transformation of raw data (fastq files) to transcript counts (quants.sf files).

The quantification software of choice is Salmon.

As of Jan 2022, the reference genome used is Homo_sapiens/NCBI/GRCh38.

Processing involves the following steps:

  • Raw fastq files uploaded to Synapse by researcher in a folder with name format experiment_name_rnaseq_fastq_date . No white space should be present in the filenames (all filenames should have _ for whitespaces. While the naming convention is a best practices recommendation and not a strict rule, the exclusion of whitespaces is required.

  • All experiment and sample related annotations need to be added on Synapse before processing can start. This is a required step so that a sample sheet can be generated to trigger the processing workflow

  • The sample sheet should contain the following information in the following format (saved as a .csv file) (More information here) :

sample

single_end

fastq_1

fastq_2

strandedness

Synapse specimenID

0 (1 if paired-end)

synID

synID

auto

 

  • The files are pulled into NextFlow workflow setup and processed using the following versions of software:

Command used to process JHU Biobank samples:

Params:

Config:

Pre-run script:

Profile: