Each sample+preparation+capture item should have a corresponding barcode with the format PROJECT-SDID-TYPE-SAMPLEID-PREPID-CAPTUREID where:
PROJECTis a two-letter short project designator. One ofAL(alascca),LB(liquid biopspy) andOT(other)SDIDis an identifier for a single individual. It must match the patternP-[a-zA-Z0-9]+(NOTE: This necessitates an additional "-" within this field).TYPEis the sample type, one ofT(tumor),N(normal) andCFDNA(ctDNA)SAMPLEIDidentifies a single biological sample, for example piece of a tumor or a single tube of plasma. It must match the pattern[a-zA-Z0-9]+.PREPIDspecifies the library preparation kit used. It must be a two-letter shortname followed by a string matching[0-9]+, which can be used to indicate the date on which the prep was performed. The date string should preferably be in the formatYYYYMMDDHHMM. For example,201701241540would indicate year 2017, January 24th, at 15:40.CAPTUREIDspecifies the capture that was performed on the library (if any). It must match eitherWGS(indicating that no capture was performed), or else a two-letter shortname indicating the capture kit used, followed by a string matching[0-9]+, which can be used to indicate the date on which the capture was performed. The date should preferably be in the formatYYYYMMDDHHMM.
NOTE: The combination SDID-TYPE-SAMPLEID must uniquely identify a single sample.
NOTE: A clinseq barcode is not garuanteed to uniquely specify a single sample+library+capture item, but in practice it should be unique if precise preparation and capture times are included within the PREPID and CAPTUREID fields.
Autoseq know about the following preparation methods:
BN=BIOO_NEXTFLEXKH=KAPA_HYPERPREPKP=KAPA_HYPERPLUSTD=THRUPLEX_DNASEQTP=THRUPLEX_PLASMASEQTF=THRUPLEX_FDTS=TRUSEQ_RNANN=NEBNEXT_RNAVI=VILO_RNA
Autoseq knows about the following capture kits:
CS=clinseq_v3_targetsCZ=clinseq_v4EX=EXOMEV3EO=EXOMEV1RF=fusion_v1CC=core_designCD=discovery_cohoCB=big_designTT=test-regionsCM=monitorCP=progression
Autoseq can use any of the runners implemented in pypedream, shellrunner (default), localqrunner or slurmrunner.
--libdir is the directory where the libraries live. Each library should have its own subdirectory where fastq.gz files can be placed. Autoseq recoginzes files on the format _1.fastq.gz/_2.fastq.gz.
The Liquid Biopsy pipeline is invoked by
autoseq --ref ref.json --outdir /path/to/outdir --jobdb jobdb.json --cores 5 --runner_name slurmrunner --libdir /path/to/libdir liqbio sample.json
The sample.json file has the format
{
"sdid": "NA12877",
"panel": {
"T": "NA12877-T-03098849-TD1-TT1",
"N": "NA12877-N-03098121-TD1-TT1",
"CFDNA": ["NA12877-CFDNA-03098850-TD1-TT1", "NA12877-CFDNA-03098850-TD2-TT1"]
},
"wgs": {
"T": "NA12877-T-03098849-TD1-WGS",
"N": "NA12877-N-03098121-TD1-WGS",
"CFDNA": ["NA12877-CFDNA-03098850-TD1-WGS"]
}
}
In this file, a single tumor and normal sample is allowed, but multiple plasma samples. If no tumor or normal sample is avaialble, they can be set to null, but if no plasma samples are available, it should be set to [] (empty list), for example "CFDNA": [].
For the plasma samples, merging of libraries will take place before calling. On alignment, the @RG tag will be set as follows:
ID=SDID-TYPE-SAMPLEID-PREPID-CAPTUREIDLB=SDID-TYPE-SAMPLEID-PREPIDSM=SDID-TYPE-SAMPLEID
Of note is that the library tag (LB) does not include the CAPTUREID part, to ensure that PCR duplicates are removed correctly.
If a single prepared samples is exposed to capture twice, to create the libraries NA12877-T-49-TD1-TT1 and NA12877-T-49-TD1-TT2 (note different digits in the capture id), read pairs being identical between the two libraries should be considered duplicates since the sample was split after the final PCR step. Therefore, the LB for these libraries is set to NA12877-T-49-TD1. After merging the bam files, removal of PCR duplicates is done using Picard MarkDuplicates, which will do the right thing.
For automated testing, a test reference genome and a test datas set with relevant data are supplied.
The test reference genome and assets is available for download at https://export.uppmax.uu.se/b2010040/test-genome.tar.gz. This archive contains a sliced version of a full set of genome files for autoseq, including various key genes.
The whole chromosomes 3, 10, 17, X and Y are selected, after which everything except the following regions have been masked (to speed up alignment):
3 178863388 179014224 PIK3CA_150k
10 83068546 96283182 PTEN_13M
17 7558477 7589399 TP53_30k
X 66782057 66796840 14k_AR_exon
Y 6810425 6825985 15k_on_Y
From these regions, key exons and various other regions have been selected to mimic a small exome.
A sythetic tumor/normal/plasma dataset has been created for testing purpuses. From the illumina platinum 200x WGS sample from NA12877, read pairs from the seleted targets have been extracted. These reads have then been randomly assigned to create a virtual normal sample with ≈50x coverage, and remaining reads (≈150x coverage) have been put aside. To create a virtual tumor and a virtual plasma sample, variants have been spiked into the 150x data in the following positions:
- TP53 insertion: MU2185182, chr17:g.7578475->G
- TP53 deletion: MU25947, chr17:g.7577558G>-
- TP53 DNV: MU52971976, chr17:g.7574003GG>AA
- PIK3CA hotspot E545K, MU5219, chr3:g.178936091G>A
- PTEN hotspot R130Q, MU29098, chr10:g.89692905G>A
- PTEN hotspot R233*, MU589331, chr10:g.89717672C>T
- AR intron variant, MU50988553, chrX:g.66788924G>A
In the virtual tumor, the target variant allele fraction (VAF) is 30% and in the virtual plasma sample the target VAF is 20%.
The variants have been selected from ICGC simple somatic mutations v20 with the aim to cover common small variants, including SNVs, deletions, insertions and DNVs. Note that the tests does not address the issue of global sensitivity and PPV of the pipeline, but are only intented to ensure that variants of all kinds are detected by the pipeline.