Troubleshooting

Software

- Open the log file ./<AnalysisFolder>/Logs_Intermediates/pipeline_trace.txt. This log file displays each pipeline step run by the Nextflow workflow manager software. If a step fails, it is marked as FAILED. Each step generates log files that are stored in step-specific subfolders in the Logs_Intermediates folder. Review the log files in the relevant Logs_Intermediates folder for the step to identify potential sources of error. - Open the errors folder ./<AnalysisFolder>/errors. The workflow creates an error file, error_<NameOfFailedStep>.json, for each step that failed during analysis. For steps that fail per sample, there is a separately labeled file for each sample that failed each step error_<NameOfFailedStep>_<SampleIDIfRelevant>.json. These files contain the command and stdout and stderr from the step.

Samples

Open the combined metrics output results file ./<AnalysisFolder>/Results/<PairId>/MetricsOutput.tsv. If a sample fails an analysis step, the Pair ID that contains the sample shows the failure under FAILED_STEPS in the Analysis Status section, and COMPLETED_ALL_STEPS shows as False. If available, review the individual log files for the failed steps under ./<AnalysisFolder>/Logs_Intermediates to identify potential sources of error.

Multinode Gather

If the following error appears, check if the sample or pair ID was included multiple times during separate node analysis runs, before being gathered together. If the error exists, rerun one of the analyses without the duplicate and reattempt gathering. ERROR:Gather:Destination file ... already exists - check if the same sample ID is in multiple input folders

Sample Sheet not found

Verify that SampleSheet.csv is present at the top level of the run folder with the name "SampleSheet.csv". If the sample sheet is in a different location, supply the sample sheet using the --sampleSheet option

Indexes are not valid for the sequencer and/or assay

See Valid indexes for assay and instrument combinations for correct indexes for the sequencer and assay.

Pair_ID is not unique

Pair_ID column is required in the TSO500S_Data section of the sample sheet, which pairs at most one RNA and one DNA sample together for analysis. If the sample does not have a pair, use a unique pair ID for single samples.

Sample Sheet is not in v2 format

Verify that the format of the sample sheet is v2. v1 sample sheet is not compatible with DRAGEN TruSight Oncology 500 Analysis Software.

Analysis does not run

Verify the analysis starts from the run folder, and BCLs or FASTQs are in the correct locations as outlined in Starting From BCL Files and Starting From FASTQ Files respectively.

TSO 500

• UP1-UP16

• CP1-CP16 (DNA Only)

TSO 500 HT

• UDP0001–UDP0192

Lane Column without Values

Ensure that the column is completed. If lane is not applicable to the run, delete the column.

Format of v2 sample sheet is incorrect

Verify that the following sections and fields are present in the sample sheet and follow the individual rules in Sample Sheet Requirements [BCLConvert_Settings] - SoftwareVersion - AdapterRead1 - AdapterRead2 - AdapterBehavior - MinimumTrimmedReadLength - MaskShortReads [BCLConvert_Data] - Sample_ID - index - index2 [TS0500S_Data] - Sample_ID - Index_ID - Sample_Type - Pair_ID - Sample Feature (Optional)

HRD analysis is missing

Verify that HRD is in the Sample Feature column in the sample sheet. Refer to Sample Sheet Requirements for more information.

Sample_ID and/or Sample_Type is not present

Verify that the sample sheet has columns and values for Sample_ID and Sample_Type.

Unique sample IDs

Verify that the Sample_IDs are unique in the sample sheet.

Format of v2 Sample Sheet is incorrect

Verify that the following sections and fields are present in the sample sheet and follow the individual rules in Sample Sheet Requirements. [TS0500S_Data] - Sample_ID - Index_ID - Sample_Type - Pair_ID

- Sample Feature (Optional) Verify when FASTQs were generated using the HRD add-kit (Not available in Japan), Sample Feature is added to those DNA Samples. Refer to Sample Sheet Requirements for more information.

Incorrect folder structure

Verify that the FASTQ files are in the correct structure. Refer to Starting From FASTQ Files for more information.

Invalid FASTQ input files

If the FASTQs are invalid, start TSO 500 analysis from BCL files.

HRD analysis missing

Make sure that HRD is in the correct column in the sample sheet.

The output file directory contains information from previous analyses

If this issue is seen: specify a new target output folder and repeat analysis To prevent this issue: specify an empty directory before starting analysis

Single exon (single probe) genes are still reported in the CNV VCF file, but not the CNV TSV file

No action needed; software is working as expected.

Currently all single probe genes are not emitted to the Copy Number Variants section of our CombinedVariantOutput.tsv. However, you can still find these events in the cnv.vcf.gz.

Due to the single probe nature, accurate CNV calling has not been validated and as such they are emitted as REF

Failure type: ValueError: Could not find pipeline ID for app BCLConvert in sample sheet SampleSheet.csv

Action: Ensure StartsFromFastq field is in the [TSO500S_Settings] section, and it is not present in the [BCLConvert_Settings] Section. Refer to Sample Sheet Requirements for more information.