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• Introduction
  • The concept of Biomedical Genomics Analysis plugin
  • System requirements
  • Contact information
• QIAseq Panel Analysis
  • Data management
  • The Analyze QIAseq Panels guide
    • Import your reads
    • Start a QIAseq panel analysis
  • How to create a custom panel analysis workflow
    • Import QIAGEN Primers
  • Create a custom Trim adapter list (optional)
• Targeted DNA
  • The Identify QIAseq DNA Variants ready-to-use workflows
    • Output from the Identify QIAseq DNA Variants workflow
    • Quality Control for the Identify QIAseq DNA Variants workflow
  • Targeted DNA tools detailed description
    • Remove and Annotate with Unique Molecular Index
    • Calculate Unique Molecular Index Groups
    • Create UMI Reads
    • Remove Ligation Artifacts
    • Trim Primers of Mapped Reads
    • Annotate Variants with Unique Molecular Index Info
    • Prepare Guidance Variant Track
• Targeted RNAscan
  • The Detect QIAseq RNAscan Fusions ready-to-use workflow
    • Output from the Detect QIAseq RNAscan Fusions workflow
    • Interpretation of the Detect QIAseq RNAscan Fusions results
  • Targeted RNAscan tools detailed description
    • Detect Fusion Genes
    • Refine Fusion Genes
    • Annotate Fusions with Known Fusion Information
    • QC for RNAscan Panels
    • Import Known Fusion Information Track
• Targeted RNA
  • The Quantify QIAseq RNA Expression ready-to-use workflow
    • Output from the Quantify QIAseq RNA Expression workflow
  • Targeted RNA tools detailed description
    • The Quantify QIAseq RNA tool
• QCI Interpret Integration
  • Configuration of the Upload to QCI Interpret tool
  • The Upload to QCI Interpret tool
• QIAGEN GeneRead DNA Panel Analysis
  • The QIAGEN GeneRead Panel Analysis workflow
    • Output from the QIAGEN GeneRead Panel Analysis
  • Trim Primers and their Dimers of Mapped Reads
• Ready-to-use workflows descriptions and guidelines
  • General Workflow
  • Somatic Cancer
  • Hereditary Disease
• Getting started
  • Import sequencing data
  • Prepare Raw Data
• Whole genome sequencing (WGS)
  • General Workflows (WGS)
    • Annotate Variants (WGS)
    • Identify Known Variants in One Sample (WGS)
  • Somatic Cancer (WGS)
    • Filter Somatic Variants (WGS)
    • Identify Somatic Variants from Tumor Normal Pair (WGS)
    • Identify Variants (WGS)
  • Hereditary Disease (WGS)
    • Filter Causal Variants (WGS-HD)
    • Identify Causal Inherited Variants in Family of Four (WGS)
    • Identify Causal Inherited Variants in Trio (WGS)
    • Identify Rare Disease Causing Mutations in Family of Four (WGS)
    • Identify Rare Disease Causing Mutations in Trio (WGS)
    • Identify Variants (WGS-HD)
• Whole exome sequencing (WES)
  • General Workflows (WES)
    • Annotate Variants (WES)
    • Identify Known Variants in One Sample (WES)
  • Somatic Cancer (WES)
    • Filter Somatic Variants (WES)
    • Identify Somatic Variants from Tumor Normal Pair (WES)
    • Identify Variants (WES)
    • Identify and Annotate Variants (WES)
  • Hereditary Disease (WES)
    • Filter Causal Variants (WES-HD)
    • Identify Causal Inherited Variants in Family of Four (WES)
    • Identify Causal Inherited Variants in Trio (WES)
    • Identify Rare Disease Causing Mutations in Family of Four (WES)
    • Identify Rare Disease Causing Mutations in Trio (WES)
    • Identify Variants (WES-HD)
    • Identify and Annotate Variants (WES-HD)
• Targeted amplicon sequencing (TAS)
  • General Workflows (TAS)
    • Annotate Variants (TAS)
    • Identify Known Variants in One Sample (TAS)
  • Somatic Cancer (TAS)
    • Filter Somatic Variants (TAS)
    • Identify Somatic Variants from Tumor Normal Pair (TAS)
    • Identify Variants (TAS)
    • Identify and Annotate Variants (TAS)
  • Hereditary Disease (TAS)
    • Filter Causal Variants (TAS-HD)
    • Identify Causal Inherited Variants in Family of Four (TAS)
    • Identify Causal Inherited Variants in Trio (TAS)
    • Identify Rare Disease Causing Mutations in Family of Four (TAS)
    • Identify Rare Disease Causing Mutations in Trio (TAS)
    • Identify Variants (TAS-HD)
    • Identify and Annotate Variants (TAS-HD)
• Whole Transcriptome Sequencing (WTS)
  • Annotate Variants (WTS)
  • Compare Variants in DNA and RNA
  • Identify Candidate Variants and Genes from Tumor Normal Pair
  • Identify Variants and Add Expression Values
  • Identify and Annotate Differentially Expressed Genes and Pathways
• Batching workflows
• Appendices
  • Legacy tools
    • Trim Primers of Mapped Single Reads
    • Trim Primers of Mapped Paired End Reads
  • Install and uninstall plugins
    • Install
    • Uninstall
• Bibliography

Subsections

• Run the Identify Causal Inherited Variants in a Family of Four (WGS) workflow
• Output from the Identify Causal Inherited Variants in a Family of Four (WGS) workflow

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Identify Causal Inherited Variants in Family of Four (WGS)

As the name of the workflow implies, you can use the Identify Causal Inherited Variants in a Family of Four (WGS) ready-to-use workflow to identify inherited causal variants in a family of four. The family of four consists of an affected child, its parents, including one affected by the condition, and one additional affected family member where (sibling, grand parent, uncle or the like).

Run the Identify Causal Inherited Variants in a Family of Four (WGS) workflow

To run the Identify Causal Inherited Variants in a Family of Four (WGS) workflow, go to:

        Toolbox | Ready-to-Use Workflows | Whole Genome Sequencing () | Hereditary Disease () | Identify Causal Inherited Variants in a Family of Four (WGS) ()

1. Double-click on the Identify Causal Inherited Variants in a Family of Four (WGS) tool to start the analysis. If you are connected to a server, you will first be asked where you would like to run the analysis.

2. The sequencing reads from the different family members are specified one at a time in successive dialogs (figure 10.33).

   
   Figure 10.33: Specify the sequencing reads for the appropriate family member.

3. Select which reference data set should be used to identify causal inherited variants (figure 10.34).

   
   Figure 10.34: Choose the relevant reference Data Set to identify causal inherited variants.

4. Specify the Hapmap populations that should be used for filtering out variants found in the Hapmap database (figure 10.35).

   
   Figure 10.35: Select the relevant Hapmap population(s).

5. Similarly, specify the parameters for the Fixed Ploidy Variant Detection tool for each family member successively (figure 10.36).

   The parameters used by the Fixed Ploidy Variant Detection tool can be adjusted. We have optimized the parameters to the individual analyses, but you may want to tweak some of the parameters to fit your particular sequencing data. A good starting point could be to run an analysis with the default settings.

   
   Figure 10.36: Specify the parameters for the Fixed Ploidy Variant Detection tool.

   The parameters that can be set are:

   • Required variant probability is the minimum probability value of the 'variant site' required for the variant to be called. Note that it is not the minimum value of the probability of the individual variant. For the Fixed Ploidy Variant detector, if a variant site - and not the variant itself - passes the variant probability threshold, then the variant with the highest probability at that site will be reported even if the probability of that particular variant might be less than the threshold. For example if the required variant probability is set to 0.9 then the individual probability of the variant called might be less than 0.9 as long as the probability of the entire variant site is greater than 0.9.
   • Ignore broken pairs: When ticked, reads from broken pairs are ignored. Broken pairs may arise for a number of reasons, one being erroneous mapping of the reads. In general, variants based on broken pair reads are likely to be less reliable, so ignoring them may reduce the number of spurious variants called. However, broken pairs may also arise for biological reasons (e.g. due to structural variants) and if they are ignored some true variants may go undetected. Please note that ignored broken pair reads will not be considered for any non-specific match filters.
   • Minimum coverage: Only variants in regions covered by at least this many reads are called.
   • Minimum count: Only variants that are present in at least this many reads are called.
   • Minimum frequency: Only variants that are present at least at the specified frequency (calculated as 'count'/'coverage') are called.

6. In the last wizard step you can check the selected settings by clicking on the button labeled Preview All Parameters. In the Preview All Parameters wizard you can only check the settings, and if you wish to make changes you have to use the Previous button from the wizard to edit parameters in the relevant windows.

7. Choose to Save your results and click on the button labeled Finish.

Output from the Identify Causal Inherited Variants in a Family of Four (WGS) workflow

The following outputs are generated:

• Reads Tracks One for each family member. The reads mapped to the reference sequence.
• Variants in ... One track for each family member. The variants identified in each of the family members. The variant track can be opened in table view to see all information about the variants.
• Putative Causal Variants in Child The putative disease-causing variants identified in the child. The variant track can be opened in table view to see all information about the variants.
• Gene List with Putative Causal Variants Gene track with the identified putative causal variants in the child. The gene track can be opened in table view to see the gene names.
• Target Region Coverage Report One for each family member. The report consists of a number of tables and graphs that in different ways provide information about the mapped reads from each sample.
• Target Region Coverage One track for each individual. When opened in table format, it is possible to see a range of different information about the targeted regions, such as target region length, read count, and base count.
• An Amino Acid Track Shows the consequences of the variants at the amino acid level in the context of the original amino acid sequence. A variant introducing a stop mutation is illustrated with a red amino acid.
• Track List This is a collection of tracks shown together in a view that makes it easy to compare information from the individual tracks, such as compare the identified putative causal variants with the read mappings and information from databases.

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