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  • seqtk安装和使用

    Installation:

    Just to cover the 'how to obtain the code' part. You will need to have git installed need to clone the seqtk url:
    git clone https://github.com/lh3/seqtk.git 
    

    then switch to the seqtk directory and make it:

    cd seqtk
    make
    

    Now you can invoke it as such:

    ~/mypath/to/seqtk/seqtk

    Usage:
    • Convert FASTQ to FASTA:

      seqtk seq -a in.fq.gz > out.fa
      
    • Convert ILLUMINA 1.3+ FASTQ to FASTA and mask bases with quality lower than 20 to lowercases (the 1st command line) or to N (the 2nd):

      seqtk seq -aQ64 -q20 in.fq > out.fa
      seqtk seq -aQ64 -q20 -n N in.fq > out.fa
      
    • Fold long FASTA/Q lines and remove FASTA/Q comments:

      seqtk seq -Cl60 in.fa > out.fa
      
    • Convert multi-line FASTQ to 4-line FASTQ:

      seqtk seq -l0 in.fq > out.fq
      
    • Reverse complement FASTA/Q:

      seqtk seq -r in.fq > out.fq
      
    • Extract sequences with names in file name.lst, one sequence name per line:

      seqtk subseq in.fq name.lst > out.fq
      
    • Extract sequences in regions contained in file reg.bed:

      seqtk subseq in.fa reg.bed > out.fa
      
    • Mask regions in reg.bed to lowercases:

      seqtk seq -M reg.bed in.fa > out.fa
      
    • Subsample 10000 read pairs from two large paired FASTQ files (remember to use the same random seed to keep pairing):关键是可以实现随机抽取序列

      seqtk sample -s100 read1.fq 10000 > sub1.fq
      seqtk sample -s100 read2.fq 10000 > sub2.fq
    • Trim low-quality bases from both ends using the Phred algorithm:

      seqtk trimfq in.fq > out.fq
      
    • Trim 5bp from the left end of each read and 10bp from the right end:

      seqtk trimfq -b 5 -e 10 in.fa > out.fa
     
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  • 原文地址:https://www.cnblogs.com/Datapotumas/p/6306192.html
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