Quality Control
The software calculates several quality control metrics for runs and samples.
Run QC
The Run Metrics section of the metrics output report provides sequencing run quality metrics along with suggested values to determine if they are within an acceptable range. The overall percentage of reads passing filter is compared to a minimum threshold. For Read 1 and Read 2, the average percentage of bases ≥ Q30, which gives a prediction of the probability of an incorrect base call (Q‑score), are also compared to a minimum threshold. The following tables show run metric and quality threshold information for different systems.
The values in the Run Metrics section are listed as NA in the following situations:
If the analysis was started from FASTQ files.
If the analysis was started from BCL files and the InterOp files are missing or corrupt.
NextSeq 500/550 or NextSeq 550Dx (RUO)
PCT_PF_READS (%)
Total percentage of reads passing filter.
≥80.0
All
PCT_Q30_R1 (%)
Percentage of Read 1 reads with quality score ≥ 30.
≥80.0
All
PCT_Q30_R2 (%)
Percentage of Read 2 reads with quality score ≥ 30.
≥80.0
All
NovaSeq 6000 or NovaSeq 6000Dx (RUO)
PCT_PF_READS (%)
Total percentage of reads passing filter.
≥55.0
All
PCT_Q30_R1 (%)
Percentage of Read 1 reads with quality score ≥ 30.
≥80.0
All
PCT_Q30_R2 (%)
Percentage of Read 2 reads with quality score ≥ 30.
≥80.0
All
NextSeq 1000/2000
PCT_PF_READS (%)
Total percentage of reads passing filter.
≥85.0
All
PCT_Q30_R1 (%)
Percentage of Read 1 reads with quality score ≥ 30.
≥85.0
All
PCT_Q30_R2 (%)
Percentage of Read 2 reads with quality score ≥ 30.
≥85.0
All
NovaSeq X
PCT_Q30_R1 (%)
Percentage of Read 1 reads with quality score ≥ 30.
≥85.0
All
PCT_Q30_R2 (%)
Percentage of Read 2 reads with quality score ≥ 30.
≥85.0
All
DNA Sample QC
DRAGEN TruSight Oncology 500 uses QC metrics to assess the validity of analysis for DNA libraries that pass contamination quality control. If the library fails one or more quality metrics, then the corresponding variant type or biomarker is not reported, and the associated QC category in the report header displays FAIL. Additionally, a companion diagnostic result may not be available if it relies on QC passing for one or more of the following QC categories.
DNA library QC results are available in the MetricsOutput.tsv
file. Refer to Metrics Output for details.
CONTAMINATION_SCORE
The contamination score is based on VAF distribution of SNPs.
Contamination Score ≤
All
MEDIAN_EXON_COVERAGE
Median exon fragment coverage across all exon bases.
≥ 150
Small variant TMB
PCT_EXON_50X
Percent exon bases with 50x fragment coverage.
≥ 90.0
Small variant TMB
MEDIAN_INSERT_SIZE
The median fragment length in the sample.
≥ 70
Small variant TMB
USABLE_MSI_SITES
The number of MSI sites usable for MSI calling.
≥ 40
MSI
MEDIAN_BIN_COUNT_CNV_TARGET
The median raw bin count per CNV target.
≥ 1.0
CNV
RNA Sample QC
The input for RNA Library QC is RNA alignment. Metrics and guideline thresholds can be found in the MetricsOutput.tsv
file. Refer to Metrics Output for details.
MEDIAN_CV_GENE_500X
The median CV for all genes with median coverage > 500x. Genes with median coverage > 500x are likely to be highly expressed. Higher CV median > 500x indicates an issue with library preparation (poor sample input and/or probes pulldown issue).
Fusion Splice
MEDIAN_INSERT_SIZE
The median fragment length in the sample.
≥ 80
Fusion Splice
TOTAL_ON_TARGET_READS
The total number of reads that map to the target regions.
≥ 9000000
Fusion Splice
GENE_MEDIAN_COVERAGE
The median deduped coverage across all genes in the RNA panel (55 genes).
N/A*
Fusion Splice
To avoid failing RNA samples unnecessarily, Illumina does not recommend a universal threshold to determine RNA sample quality. RNA expression varies significantly across tissue types and a small panel size (55 genes), which makes normalization challenging. Tissue-specific thresholds could be considered for normalization.
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