Question

Trouble with transcriptome data

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7.1 years ago

gayachit ▴ 200

Hi everyone

I have 14 Gb of transcriptome data of a plant sequences using Ion Proton. Initially I ran a quality assessment tool for checking it and there are a lot of overrepresented sequence probably rRNA. When I try to use fastq_quality_filter to remove low quality bases it gives me an error "Invalid quality score on line 210650840 [quality tok >:::;998;;::;5;;5<<18:;<<<=?7<;;;;;;<<==?;;;5;;299;::"

I tried searching for similar posts. Now m thinking whether to remove the whole read or not. Please suggest what can be done

RNA-Seq next-gen Ion Proton • 1.3k views

ADD COMMENT • link updated 7.1 years ago by Benn 8.3k • written 7.1 years ago by gayachit ▴ 200

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Please chose a more informative title and add relevant tags, such as ion proton

ADD REPLY • link 7.1 years ago by WouterDeCoster 47k

score 0 · Answer 1 · 2017-03-23

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7.1 years ago

gangireddy ▴ 160

Hi gayachit,

This is a naive answer. But here it goes :

It will not affect your data if remove a single read.

and generally the first few bases of most sequencing reads have poor qualities and they need to be chopped off.

so, you can try chopping of first few bases.

ADD COMMENT • link 7.1 years ago by gangireddy ▴ 160

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Thanks gangreddy Those bases were at the end of my file. So i removed them

ADD REPLY • link 7.1 years ago by gayachit ▴ 200

score 0 · Answer 2 · 2017-03-23

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7.1 years ago

Benn 8.3k

You'll probably have to set the phred score parameter to -Q33.

ADD COMMENT • link 7.1 years ago by Benn 8.3k

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-Q33 didn't work. I tried that earlier... But thanks anyway

ADD REPLY • link 7.1 years ago by gayachit ▴ 200

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Okay, it would be helpful if you explained already what you have tried. Or present some code, just an idea.

ADD REPLY • link 7.1 years ago by Benn 8.3k