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DRAGEN Protein Quantification
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DRAGEN Protein Quantification
  • Get Started
    • Introduction
    • Prerequisites
      • Illumina Protein Prep Automation System Output Files
  • Run Setup
    • Run Planning with the BSSH Run Planner Tool
    • Sample Sheet Fields
    • Local Sample Sheet Generation Tool
    • Lane Splitting and Multi-Analysis by Project
  • Counting and Normalization
    • Cloud Autolaunch Secondary Analysis
      • Accessing Cloud Results
    • Local Secondary Analysis
    • Normalization Summary
    • QC Summary
    • Interpretation of Results
    • Metrics Appendix
  • Output Files
    • Output Structure
    • DRAGEN Report
    • ADAT Content
  • After Counting and Normalization
    • Using the ADAT
    • Illumina Connected Multiomics Walkthrough
  • References
    • FAQs
    • Documentation Revision History
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  • Process FAQs
  • Metrics and Results FAQs

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  1. References

FAQs

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Last updated 1 month ago

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Process FAQs

  • How can I share data with a collaborator in BSSH?

    • See the following documentation:

  • I sequenced in manual mode/need to kick of autolaunch after sequencing is complete. How can I do this?

    • Use the BSSH CLI to upload the run folder to BSSH. Make sure the samplesheet is named "SampleSheet.csv" and you are using an up-to-date version of the tool - at least v1.6.1.

    • For additional information, see the following documentation:

  • How do I download/export the samplesheet?

    • Go to the BSSH Run Planner:

      • Go to BSSH, select the intended workgroup on the top right, and then select the Runs tab

      • Additional information on the BSSH Run Planner:

    • For a new run:

      • Select the "New Run" button on the right and plan a new run with the desired pipeline.

      • After ingesting the IPPAS output files in the BSSH Run Planner, the user will reach the following Run Review page:

      • Select the "Export" option on the bottom right to download the samplesheet created

      • Select the "Save as Draft" or "Save as Planned" options to save this run as a draft or planned run respectively\

    • For an "Active" or "Planned" run:

      • Select the intended tab mentioned under the Runs header.

      • Select the required run from the list of runs:

      • Next, click File > Download > Sample Sheet:

  • How can I requeue a run on BSSH with a new samplesheet/new version of the pipeline?

    • Go to the BSSH Run Planner tool and plan a new run with the desired pipeline.

    • Save the exported samplesheet (see the above step for additional information).

    • Go to the original run, and click Status > Requeue > Planned Run.

    • Select "Use a new Sample Sheet".

    • Upload the new sample sheet.

    • On the next page, click "requeue".

  • Can multi-analysis by project split samples on the same plate?

    • No. All samples on the same plate must have the same project.

Metrics and Results FAQs

  • What is DRC_Level and why is this used?

    • DRC stands for Dynamic Range Compression. It is used to even out the SOMAmer concentrations from a 5-log dynamic range to 2-log. Without DRC, the most abundant SOMAmers would occupy the majority of sequencing readout capacity. Each sample would require extremely high sequencing depth to cover the unabundant SOMAmers and accurately quantify them. In using DRC, probes are grouped based on their observed abundances under no DRC condition, and each group is compressed by a different set ratio. The compression level of each SOMAmer is included in the DRC_Level row of SOMAmer metadata.

  • What is the LoD, and what does it indicate?

    • LoD stands for Limit of Detection. Each SOMAmer has an LoD for both Plasma and Serum. The LoD is a noise floor for that SOMAmer's fully normalized (MedNormExt) counts. In other words, normalized counts above the SOMAmer's LoD reflect the relative abundance of that SOMAmer's target protein, whereas normalized counts below its LoD may reflect assay uncertainty.

  • How should LoD be used to discern signal?

    • The normalized count of a given protein is considered signal if it is above the LoD for that protein for it's given sample type.

  • How do Somalogic and Illumina metrics compare?

    • Metrics and Normalization steps with different names between Somalogic's tool and Illumina's DRAGEN Protein Quantification. See the table below for the approximate mapping.

Somalogic Normalization Steps
Illumina Protein Prep Normalization Steps
Notes

Raw RFU

Raw

Hyb Normalization

HybNorm

medNormInt

MedNormInt

plateScale

PlatformSpecificPlateScale

Calibration

PlatformSpecificCalibrate

-

CrossPlatformPlateScale,

Applied to normalize data across instruments

-

CrossPlatformCalibrate

Applied to normalize data across instruments

-

MedNormExt

anmlQC

-

qcCheck

QCCheck

anmlSMP

-

Filtered

-

  • Where are the FASTQs?

    • DRAGEN Protein Quantification does not produce FASTQs. By utilizing DRAGEN Counting, the software uses BCL Convert to demultiplex and count proteins per sample at the same time. This reduces analysis time but also removes FASTQ as a pipeline output.

  • What if the PF or Q30 values are lower than expected?

    • First, check secondary metrics. If secondary metrics are passing, it's acceptable to proceed with further analysis. If secondary metrics have warnings or failures, consider re-pooling or repeating the dilute and denature and sequencing of the saved pool. If the data still looks poor, reach out to tech support for further guidance.

  • What organisms does the SOMAmer metadata cover in the 9.5k assay?

Organism
# of SOMAmers in the 9.5 Assay

Human

10326

Mouse

230

Gila monster

3

Hornet

3

Jellyfish

3

African clawed frog

3

Thermus thermophilus

3

European elder

2

Common eastern firefly

2

E. coli

1

HIV-1

1

HIV-2

1

Bacillus stearothermophilus

1

Ensifer meliloti

1

Red alga

1

https://help.connected.illumina.com/basespace-sequence-hub/collaborate/share-with-collaborators
https://help.connected.illumina.com/basespace-sequence-hub/cmd-line-interfaces/basespace-cli
https://help.basespace.illumina.com/sequence/plan-runs