How to change the quality score of reads ? (quick help is appreciated)
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8.7 years ago
mbparsa ▴ 10

So I have my FASTQ ran through Tophat and produced unmapped and mapped bam files, I would like to increase the quality score for all mapped sequences, and then use TopHat to remap them, What is the easiest and best way of doing it?

RNA-Seq BAM Tophat FASTQ • 3.4k views
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Why do you want to do this? One should never change primary data (or at least not without a good reason).

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It is only an experiment, to see how it is gonna affect the result ? can you kind of predict what would be the result ?

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If a read has already aligned that alignment would not change by changing the Q-score.

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Exactly, only if TopHat is working as expected !

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8.7 years ago
chen ★ 2.5k

If you are able to use Julia (http://julialang.org/), you can use OpenGene (https://github.com/OpenGene/OpenGene.jl) to do this easily

Following code is tested:

using OpenGene

# no quality can be higher than K
const QUAL_LIMIT = 'K'
# how much you want to increase it
const QUAL_INC = 10

# R1.fq is the file name of your fastq
istream = fastq_open("R1.fq")
ostream = fastq_open("R1.out.fq","w")

# fastq_read will return an object FastqRead {name, sequence, strand, quality}
# fastq_write can write a FastqRead into a ouput stream
while (fq = fastq_read(istream))!=false
    qual_arr = [q for q in fq.quality.qual]
    for i in 1:length(qual_arr)
        qual_arr[i] = min(qual_arr[i]+QUAL_INC, QUAL_LIMIT)
    end
    fq.quality.qual = ASCIIString(qual_arr)
    fastq_write(ostream, fq)
end

close(ostream)

You can install Julia by sudo apt-get install julia if you are running Ubuntu, after you install it, just change the file names in the code, launch julia, paste the code and press ENTER.

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Thanks, so your suggesting to first convert it to a "FASTQ" file (I am assuming tools like bedtools) and then manipulate it from there? I dont have Julia but I can use Matlab to do the same thing you are suggesting. My last question would be: you are converting ASCII to integer and add 10 to it ? can I ask why 10 ?

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10 is a parameter, you can use any other number.

By adding 10, Q20 will become Q30, if you use 5, it will become Q25, all up to you.

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You have fastq files that you used for tophat alignment so the code above would take them as input. No conversion should be needed.

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so the reason that I am doing this is I would like to increase the score only for the "mapped alignment" what would you recommend?

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I see. You could use fastq command from samtools to get the fastq reads. You may need to How To Filter Mapped Reads With Samtools before doing the conversion.

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I installed julia on my Fedora machine and just paste the code which was mentioned above. I get this error " ERROR: UndefVarError: fastq_open not defined ". So kindly help.

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7.4 years ago
madhu.9124 ▴ 60

I installed julia on my Fedora machine and just paste the code which was mentioned above. I get this error " ERROR: UndefVarError: fastq_open not defined ". So kindly help.

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Use ADD COMMENT/ADD REPLY when responding to existing posts to keep threads logically organized. SUBMIT ANSWER should only be used for new answers for the original question.

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