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• Introduction
  • The concept of CLC Microbial Genomics Module
  • Contact information
• System requirements and installation
  • System requirements
  • Installation of modules
  • Licensing modules
  • Uninstalling modules
  • Server License
• Introduction to Metagenomics
• De Novo Assemble Metagenome
• Amplicon-Based Analysis
  • Normalize OTU Table by Copy Number
  • Filter Samples Based on Number of Reads
  • OTU clustering
    • OTU clustering parameters
    • OTU clustering tool outputs
    • Visualization of OTU abundance tables
    • Create taxonomic level subtables for heat maps
    • 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
  • Identify Viral Integration Sites
    • The Viral Integration Viewer
    • The Viral Integration Report
  • Workflows
    • Analyze Viral Hybrid Capture Panel Data
    • 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
• 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
  • Extend Result Metadata Table
  • Add to Result Metadata Table (legacy)
  • Use Genome as Result
• Workflow templates
  • Map to Specified Reference
    • How to run the Map to Specified Reference workflow
  • Type Among Multiple Species
    • Preliminary steps to run the Type Among Multiple Species workflow
    • How to run the Type Among Multiple Species workflow
    • Example of results obtained using the Type Among Multiple Species workflow
  • Type a Known Species
    • Preliminary steps to run the Type a Known Species workflow
    • How to run the Type a Known Species workflow
    • Example of results obtained using the Type a Known Species workflow
  • Extract Regions from Tracks
  • Create Large MLST Scheme with Sequence Types
  • Compare Variants Across Samples
• Find the best matching reference
  • Find Best Matches using K-mer Spectra
  • From samples best matches to a common reference for all
  • Find Best References using Read Mapping
    • The Find Best References using Read Mapping Report
• 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
• Large MLST Scheme Tools
  • Getting started with the Large MLST Scheme tools
  • Large MLST Scheme Visualization and Management
  • Minimum Spanning Trees
    • The Minimum Spanning Tree view
    • Navigating the Tree view
    • The Layout panel
    • The Metadata panel
  • Type With Large MLST Scheme
    • Type With Large MLST Scheme results
    • The Large MLST Typing Result element
  • Add Typing Results to Large MLST Scheme
  • Identify Large MLST Scheme from Genomes
• Functional Analysis
  • Find Prokaryotic Genes
  • Annotate with BLAST
  • Annotate with DIAMOND
  • Annotate CDS with Best BLAST Hit
  • Annotate CDS with Best DIAMOND Hit
  • Annotate CDS with Pfam Domains
  • Build Functional Profile
    • Functional profile abundance table
  • Infer Functional Profile
• Drug Resistance Analysis
  • Find Resistance with PointFinder
  • Find Resistance with Nucleotide DB
  • Find Resistance with ShortBRED
    • Resistance abundance table
• Databases for Large MLST Schemes
  • Create Large MLST Scheme
  • Download Large MLST Scheme
  • Import Large MLST Scheme
• Databases for Amplicon-Based Analysis
  • Download Amplicon-Based Reference Database
• Databases for Taxonomic Analysis
  • Download Curated Microbial Reference Database
    • Extracting a subset of a database
  • Download Custom Microbial Reference Database
    • Database Builder
  • Download Pathogen Reference Database
    • Download Pathogen Reference Database output report
  • Create Taxonomic Profiling Index
• Databases for Functional Analysis
  • Download Protein Database
  • Download Ontology Database
    • The GO Database View
    • The EC Database View
  • Create DIAMOND Index
  • Import RNAcentral Database
  • Import PICRUSt2 Multiplication Table
• Databases for Drug Resistance Analysis
  • Download Resistance Database
    • ARES Database
• QIAseq 16S/ITS Demultiplexer
• Tools
  • Split Sequence List
  • Create Annotated Sequence List
    • Examples of databases
  • Mask Low-Complexity Regions
    • Mask Low-Complexity Regions Report
• Appendices
  • Using the Assembly ID annotation
  • Legacy tools
    • Optional Merge Paired Reads
    • Fixed Length Trimming
    • MLST tools (legacy)
    • Schemes visualization and management
    • Identify MLST
    • Identify MLST Scheme from Genomes
    • Download MLST Schemes
    • Download other MLST Schemes
    • Create MLST Schemes
    • Add NGS MLST Report to Scheme
    • Merge MLST Schemes
    • Add Sequences to MLST Schemes
    • Map to Specified Reference (legacy)
      • How to run the Map to Specified Reference (legacy) workflow on a single sample
      • How to run the Map to Specified Reference (legacy) workflow on a batch of samples
    • Type among Multiple Species (legacy)
      • Preliminary steps to run the Type Multiple Species workflow
      • How to run the Type among Multiple Species (legacy) workflow
      • Example of results obtained using the Type among Multiple Species (legacy) workflow
    • Type a Known Species (legacy)
      • Preliminary steps to run the Type a Known Species (legacy) workflow
      • How to run the Type a Known Species (legacy) workflow
      • Example of results obtained using the Type a Known Species (legacy) workflow
  • Licensing requirements for the CLC Microbial Genomics Module
    • Licensing modules on a Workbench
      • 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
    • Licensing Server Extensions on a CLC Server
      • Download a static license on a non-networked machine
• Bibliography

Fixed Length Trimming

The Fixed Length Trimming tool has been moved to Legacy Tools folder because the OTU Clustering tool can now deal with reads with variable lengths. The input sequences are aligned to reference OTU sequences (e.g. the reference database) and, if the input sequence is shorter, the unaligned ends of the reference are ignored.

In previous versions of the software, in order to compare sequences and cluster them, they all needed to be of exact same length. All reads which are shorter than the cut-off were discarded, and reads longer than that were trimmed back to the chosen length.

To run the tool, go to

Toolbox | Legacy tools () | Fixed Length Trimming ()

and select the sequences you would like to trim.

In the next wizard window you can enter manually the desired length for the trimmed reads. Alternatively, the Fixed length Trimming algorithm can calculate the trimming cut-off value as the mean length of the merged reads minus one standard deviation. If this option is chosen, it is important that all samples are trimmed at the same time as the mean and standard deviation for the combined reads in all samples needs to be estimated at once.

You can also offset one adapter or barcode by typing the nucleotide sequence in the Primer offset window. Exact matching is performed but ambiguous symbols are allowed. For more than one adapter, we recommend to perform prior to the Fixed Length trimming a Trim Reads step with Automatic read-through adapter trimming. are allowed. For more than one adapter, we recommend to perform prior to the Fixed Length trimming a Trim Reads step with Automatic read-through adapter trimming.

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