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  • Raw DNA-Seq Data Processing

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  1. Input data: On this page you must input FASTQ file(s). 

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  2. Pre-processing: On this page you can modify filtration parameters. 

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    The following parameters are available :

    Base qualityQuality threshold

    for

    trimming.Reads lengthToo short

    reads

    are discarded by the filter.Trim both endsTrim the both ends of a read or not. Usually, you need to set True for Sanger sequencing and False for NGS

    and reads pairs filtration:

    for pairs  for pairs  for pairs Adapters for pairs adapter 3 The adapter itself and anything that follows is trimmed. If the adapter sequence ends with the '$ character, the adapter is anchored to the end of the read and only found if it is a suffix of the read
    Base qualityQuality threshold for trimming.
    Reads lengthToo short reads are discarded by the filter.
    Trim both endsTrim the both ends of a read or not. Usually, you need to set True for Sanger sequencing and False for NGS
    3' adapters

    Adapters

    A FASTA file with one or multiple sequences of adapter that were ligated to the 3' end. The adapter itself and anything that follows is trimmed. If the adapter sequence ends with the '$ character, the adapter is anchored to the end of the read and only found if it is a suffix of the read.

     

    5' adapters

    A FASTA file with one or multiple sequences of

     adapters that were ligated to the

     5' end.

     If the adapter sequence starts with the character ^, the adapter is 'anchored'. 

    An anchored adapter must appear in its entirety at the 5' end of the read (it is a prefix of the read). A non-anchored adapter may appear partially at the 5' end, or it may occur within the read. 

    If it is found within a read, the sequence preceding the adapter is also trimmed. In all cases, the adapter itself is trimmed.

    5' and 3' adapters A FASTA file with one or multiple sequences of adapter that were ligated to the 5' end or 3' end.
  3. Mapping: On this page you must input reference and optionally modify advanced parameters. 

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    The following parameters are available:

    Reference genomePath to indexed reference genome.
    Number of threadsNumber of threads (-t).
    Min seed lengthPath to indexed reference genome (-k).

    Band width

    Band width for banded alignment (-w).

    Dropoff

    Off-diagonal X-dropoff (-d).

    Internal seed length

    Look for internal seeds inside a seed longer than {-k} (-r).

    Skip seed threshold

    Skip seeds with more than INT occurrences (-c).

    Drop chain threshold

    Drop chains shorter than FLOAT fraction of the longest overlapping chain (-D).

    Rounds of mate rescuesPerform at most INT rounds of mate rescues for each read (-m).
    Skip mate rescueSkip mate rescue (-S).
    Skip pairingSkip pairing; mate rescue performed unless -S also in use (-P).
    Mismatch penaltyScore for a sequence match (-A).
    Mismatch penaltyPenalty for a mismatch (-B).
    Gap open penaltyGap open penalty (-O).
    Gap extention penaltyGap extension penalty; a gap of size k cost {-O} (-E).
    Penalty for clippingPenalty for clipping (-L).
    Penalty unpairedPenalty for an unpaired read pair (-U).
    Score thresholdMinimum score to output (-T).
  4. Post-processing: On this page you can modify post-processing parameters. 

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    The following parameters are available:

    MAPQ thresholdMinimum MAPQ quality score.
    Skip flagSkip alignment with the selected items. Select the items in the combobox to configure bit flag. Do not select the items to avoid filtration by this parameter.
    RegionRegions to filter. For BAM output only. chr2 to output the whole chr2. chr2:1000 to output regions of chr 2 starting from 1000. chr2:1000-2000 to ouput regions of chr2 between 1000 and 2000 including the end point. To input multiple regions use the space seprator (e.g. chr1 chr2 chr3:1000-2000).

    For single-end reads

    Remove duplicates for single-end reads.

  5. Output data: On this page you must input output parameters. 

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