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  • standard of clean data

    Hi all
    I recently got my prokaryotes RNA-seq data report back. the standard filter steps of the raw data set by our local sequencing center is as following:
    1. remove reads with adaptors
    2. remove reads with unknown nucleotides larger than 10%
    3. remove reads with low quality (more than 40% of the bases' qualities are less than 20)
    4. Obtain clean reads

    Is this suitable standard, is there any reference that discusses this topic, thanks!

  • #2
    standard of clean data

    Originally posted by Pengfei Liu View Post

    1. remove reads with adaptors
    In general, one would trim the reads to remove the adapter sequence, not remove the entire read.

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