• Product manuals

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• Introduction
• General Description
  • Supported sample kits
  • Accessing RNA-seq Analysis Portal
  • Analysis credits for RNA-seq Analysis Portal
• Getting Started
  • Upload sequencing data
  • Align and count
  • Create experiment
  • View and filter results
  • What's next - sending results to GeneGlobe
  • Next steps in GeneGlobe
• User Interface
  • Analysis Portal page
    • Front page and Projects overview
    • Project view
    • Send copy of project
  • Samples page
• Starting Analyses
  • Align and count dialog
    • QIAseq UPX 3' Transcriptiome Kit and QIAseq UPXome RNA Lib Kit specific settings
  • Create experiment dialog
    • Sample grouping
    • Experimental design
  • Compare analyses dialog
• Viewing Results
  • Experiment summary and QC report
  • Differential expression view
    • Feature table
    • Volcano plot
    • Heat map
    • Biological insights table
    • Filter
    • What's next
  • Comparison view
• RNA-seq Analysis Portal analysis explained
  • Align and count analysis workflows
    • Align and count - QIAseq miRNA Library Kit
    • Align and count - QIAseq UPX 3' Transcriptome Kit
    • Align and count - QIAseq UPXome RNA Lib Kit
    • Align and count - Demultiplexed RNA sample kits
  • Create experiment analysis workflow
  • Taxonomic profiling of unmapped reads
  • Compare analyses
• Appendix A - Sequence file naming pattern
• Appendix B - Reference and annotation information
  • General references and annotations
  • Sample kit specific resources
• Appendix C - Analysis workflow versions, species support and parameters
  • QIAseq miRNA Library Kit
  • QIAseq UPX 3' Transcriptome Kit
  • QIAseq UPXome RNA Lib Kit
  • QIAseq UPXome RNA Lib Kit (N6-T RT primer)
  • QIAseq UPXome RNA Lib Kit (ODT-T RT primer)
  • QIAseq UPXome RNA Lib Kit (N6-T + ODT-T RT primers)
  • QIAseq FastSelect RNA Lib Kit (N6-T RT primer)
  • QIAseq FastSelect RNA Lib Kit (ODT-T RT primer)
  • QIAseq FastSelect RNA Lib Kit (N6-T + ODT-T RT primers)
  • QIAseq Stranded mRNA Select/Stranded Total RNA Lib Kit
  • TruSeq Stranded Total RNA Library Prep (Human/Rat, Gold, Globin)
  • Illumina Stranded Total RNA Prep with Ribo-Zero Plus
  • NEBNext Ultra II Directional RNA Library Prep Kit for Illumina
  • KAPA RNA HyperPrep Kit
  • SMARTer Stranded Total RNA Sample Prep Kit - HI Mammalian/Low Input Mammalian
  • Collibri Stranded RNA Library Prep Kit for Illumina Systems

QIAseq UPX 3' Transcriptiome Kit and QIAseq UPXome RNA Lib Kit specific settings

The data generated with QIAseq UPX 3' Transcriptiome and QIAseq UPXome RNA Lib Kits is multiplexed, why an initial demultiplex analysis step is required. The below settings relate to this analysis step and are specific to these kits.

Custom R2 primer (QIAseq D Read 2 Primer I)

Sample Kit: QIAseq UPX 3' Transcriptiome Kit

Figure 32: The custom R2 primer setting is available for the QIAseq UPX 3' Transcriptome Kit only.

The QIAseq D Read 2 Primer I option determines which adapter list is used for demultiplexing and is essential for proper processing of the sequencing reads.

For information about the custom R2 primer, please refer to the QIAseq UPX 3' Transcriptome Handbook, available from the Product Resources tab on the QIAseq UPX 3' Transcriptiome Kit product page: https://www.qiagen.com/products/discovery-and-translational-research/next-generation-sequencing/rna-sequencing/three-rnaseq/qiaseq-upx-3-transcriptome-kits/

Well selection

Sample Kits: QIAseq UPX 3' Transcriptiome Kit, QIAseq UPXome RNA Lib Kit

This setting is sample data specific. This is why you can only analyze one QIAseq UPX 3' Transcriptiome or QIAseq UPXome RNA Lib Kit sample data item at a time.

1. If this option is available, specify whether you used a 96-well or a 384-well plate.
2. Select the wells used on the well plate in the laboratory. Make sure to select the correct wells, including considering the plate orientation. Use the checkboxes to the right of and below the wells to select an entire row or column (figure 33).

   Correct well selection is important because reads from a specific well all contain the same barcode. During demultiplexing, the first step in UPX data analysis, reads are grouped into samples based on the barcodes they carry. One sample is created per indicated barcode, i.e. per selected well. If well selection here is not identical to the actual wells used in the laboratory, the demultiplexing step will look for the wrong barcodes, leading to samples with very few or no reads.

Figure 33: Select the wells that were used on the actual well plate in the laboratory.

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