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Originally posted by maubp
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Really thanks, maubp. The problem solved~! -
The same for 500bp reads where the default is better for 0-2% error rates.Originally posted by aleferna View PostComment
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I have got somewhat related question, how do I tweak gsMapper parameters in order to get the reads mapped without introducing gaps. I am looking for SNPs and InDels and the gsMapper output (454AllDiffs.txt) shows gaps rather than mismatches. The mappings to the reference sequence looks fine, but when it comes to detecting variants the mapper is not doing what I expected it to do. Is there some extra step that I am missing for SNP/Indel detection? I have also tried AVA, but as my sequence is not an amplicon (far too big than the standard definition of amplicon in 454 terms), AVA isnt of much help either.Comment
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Hello Everybody
I would like to know if it is better to use 1 or more reference genome at a time, using the reference gs mapper, for 454 reads
Thank YouComment
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