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• Introduction
  • The concept of CLC Microbial Genomics Module
  • Contact information
• System requirements and installation
  • System requirements
  • Installation of modules
  • Plugins licenses
  • Uninstalling modules
  • Server License
• Introduction to Metagenomics
• De Novo Assemble Metagenome
• Amplicon-Based Analysis
  • Filter Samples Based on Number of Reads
  • OTU clustering
    • OTU clustering parameters
    • OTU clustering tool outputs
    • Visualization of OTU abundance tables
    • Importing and exporting OTU abundance tables
  • Remove OTUs with Low Abundance
  • Align OTUs with MUSCLE
  • Amplicon-Based Analysis Workflows
    • Data QC and OTU Clustering workflow
    • Estimate Alpha and Beta Diversities workflow
• Taxonomic Analysis
  • Contig Binning
    • Bin Pangenomes by Taxonomy
    • Bin Pangenomes by Sequence
  • Taxonomic Profiling
    • Taxonomic profiling abundance table
    • Taxonomic Profiling report
    • Sorted Reads Files
  • Workflows
    • Data QC and Clean Host DNA
    • Data QC and Taxonomic Profiling
    • Merge and Estimate Alpha and Beta diversities
    • QC, Assemble and Bin Pangenomes
• Abundance Analysis
  • Merge Abundance Tables
  • Alpha Diversity
    • Alpha diversity measures
  • Beta Diversity
    • Beta diversity measures
  • PERMANOVA Analysis
  • Differential Abundance Analysis
  • Create Heat Map for Abundance Table
  • Add Metadata to Abundance Table
  • Convert Abundance Table to Experiment
• Introduction to Typing and Epidemiology (beta)
• Handling of metadata and analysis results
  • Importing Metadata Tables
  • Associating data elements with metadata
  • Create a Result Metadata Table
  • Running an analysis directly from a Result Metadata Table
    • Filtering in Result Metadata Table
    • Filtering in a SNP-Tree creation scenario
  • Add to Result Metadata Table
  • Use Genome as Result
• Workflow templates
  • Map to Specified Reference
    • How to run the Map to Specified Reference workflow on a single sample
    • How to run the Map to Specified Reference workflow on a batch of samples
  • Type Among Multiple Species
    • Preliminary steps to run the Type Multiple Species workflow
    • How to run the Type among Multiple Species workflow for a single sample
    • Example of results obtained using the Type among Multiple Species workflow
    • How to run the Type among Multiple Species workflow on a batch of samples
  • Type a Known Species
    • Preliminary steps to run the Type a Known Species workflow
    • How to run the Type a Known Species workflow for a single sample
    • Example of results obtained using the Type a Known Species workflow
    • How to run the Type a Known Species workflow on a batch of samples:
  • Extract Regions from Tracks
• Find the best matching reference
  • Find Best Matches using K-mer Spectra
  • From samples best matches to a common reference for all
• Phylogenetic trees using SNPs or k-mers
  • Create SNP Tree
    • SNP tree output report
    • Visualization of SNP Tree including metadata and analysis result metadata
    • SNP Tree Variants editor viewer
    • SNP Matrix
  • Create K-mer Tree
    • Visualization of K-mer Tree for identification of common reference
• NGS MLST
  • Schemes visualization and management
  • Identify MLST
  • Identify MLST Scheme from Genomes
• Functional Analysis
  • Find Prokaryotic Genes
  • Annotate CDS with Best BLAST Hit
  • Annotate CDS with Best DIAMOND Hit
  • Annotate CDS with Pfam Domains
  • Build Functional Profile
    • Functional profile abundance table
• Drug Resistance Analysis
  • Find Resistance with PointFinder
  • Find Resistance with Nucleotide DB
  • Find Resistance with ShortBRED
    • Resistance abundance table
• Databases for NGS-MLST
  • Download MLST Schemes
  • Download other MLST Schemes
  • Create MLST Schemes
  • Add NGS MLST Report to Scheme
  • Merge MLST Schemes
  • Add Sequences to MLST Schemes
• Databases for Amplicon-Based Analysis
  • Download Amplicon-Based Reference Database
  • Set Up Amplicon-Based Reference Database
• Databases for Taxonomic Analysis
  • Download Microbial Reference Database
  • Set Up Microbial Reference Database
  • Download Pathogen Reference Database
    • Extracting a subset of a database
    • Download Pathogen Reference Database output report
  • Create Taxonomic Profiling Index
• Databases for Functional Analysis
  • Download Protein Database
  • Download GO Database
  • Create DIAMOND Index
• Databases for Drug Resistance Analysis
  • Download Resistance Database
    • ARES Database
  • Set Up Gene Database
• QIAseq 16S/ITS Demultiplexer
• Legacy tools
  • Optional Merge Paired Reads
  • Fixed Length Trimming
• Licensing requirements for the CLC Microbial Genomics Module
  • Workbench licenses
    • Request an evaluation license
    • Download a license using a license order ID
    • Import a license from a file
    • Configure license server connection
    • Download a static license on a non-networked computer
  • Server licenses
    • Static license installation
    • Windows license download
    • macOS license download
    • Linux license download
    • Download a static license on a non-networked machine
    • Network license installation
• Bibliography

Beta Diversity

Beta diversity examines the change in species diversity between ecosystems. The analysis is done in two steps. First, the tool estimates a distance between each pair of samples (see Beta diversity measures). Once the distance matrix is calculated, the beta diversity analysis tool performs Principal Coordinate Analysis (PCoA) on the distance matrices. These can be visualized by selecting the PCoA icon () in the bottom of the Beta Diversity results ().

If you are working with an OTU table, you can specify an appropriate phylogenetic tree for computing phylogenetic diversity. In that case, you must have aligned the OTUs and constructed a phylogeny before running the Beta Diversity tool.

To run the tool, open

        Metagenomics () | Abundance Analysis () | Beta Diversity ()

Select an abundance table with more than one sample as input (i.e., an OTU table table, or a merged functional or profiling table) and set the parameters for the beta diversity analysis as shown in figure 7.6.

Figure 7.6: Set up parameters for the Beta diversity tool.

The output of the tool is a 3D PCoA plot (figure 7.7) that can also be seen as a table or a 2D Principal Coordinate Plot.

Figure 7.7: Beta diversity results seen as a 3D PCoA, with coloring done according to the categories dedined by the metadata.

Use the settings in the right hand Side Panel of the PCoA (2D or 3D) to modify the plot visualization.

In the section Metadata, the Color menu (1) allows you to choose whether you want your data to be colored according to categorical variables (the ones defined by the metadata, as seen in figure 7.7) or by abundance values (figure 7.8).

Figure 7.8: Beta diversity results seen as a 3D PCoA, with coloring done according to taxonomic abundance values.

Coloring per abundance values is done with a gradient scheme. Click on the gradient bar to choose from several color schemes (2). Double-click on the slider to set specific values for the gradient (3).

When coloring "By abundance values", it is possible to control the abundance value calculation through existing metadata fields: Name, Taxonomy or, in the case of OTU abundance tables, Sequence. The drop down menu will then display the items that can be deselected (4) if you want to remove them from the abundance value calculation: this will not remove any of the data point from the PCoA view, but just change the abundance values of the affected point and therefore its coloring. To remove a data point from the plot, use the Show point menu (5) below in the Side Panel.

As in other metadata Side Panel features, use the field above each menu (6) to filter that menu. This is particularly helpful when menus are very long, as is the case with taxonomies for example.

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Subsections

• Beta diversity measures

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