Originally posted by mard
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if you are interested in illumina, look into fastx toolkit (link above). there's a command line tool to do it. they might also have a web interface for it, but i'm not 100% positive. the logic behind their trimming is probably good for short reads, but not as optimal for longer ones like 454.Leave a comment:
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I am unconvinced that trimming low quality reads is necessary at all. After all, most aligners (e.g., Maq, Bowtie, BWA; but not Eland!) take into account the quality score and disregard or downweight low quality reads automatically.
SimonLeave a comment:
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I don't have any perl examples, but there are some very simple Python examples in the Biopython Tutorial (search for FASTQ):
and here:
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updates on this thread?
would you suggest me a perl script for quality trimming illumina 1.3 reads?
what do you think about clc trim sequences tool? and abyss -q option?Leave a comment:
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hi .. is there any script to mask or remove the low quality repeats and also simple repeats..I would also
like to know whether this will create problems in denovo assembly...Leave a comment:
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ok, thanks for the reply. that's the impression I was getting from google.
in case anyone else reads this, i did come across this:
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Most people I've talked to use their own Perl or Python scripts for this, although EMBOSS are looking at adding this kind of tool to their suite.Leave a comment:
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Quality trimmming / Mask low quality bases?
Does anyone know of a command line utility that can accept either FASTA/QUAL or FASTQ files and mask any bases below a given quality score (ie. convert them to N)?
Does anyone have suggestions on the best utilities to perform quality score based end trimming?
Thank you for any help or suggestions.
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