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I have a FASTA file with an alignment of multiple gene samples. I am trying to develop a program that can count the number of mutations for each sample. What's the best way to do this? Store each gene sample in a dictionary and compare them somehow?

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This is a REALLY specific question... –  Wiz Sep 25 '12 at 3:59
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Perhaps a sample of your input, the unsorted version and the sorted version would help. –  Burhan Khalid Sep 25 '12 at 4:08
    
The alignment has DNA sequences that are all the same length, without any gaps. –  user1647556 Sep 25 '12 at 13:02
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2 Answers 2

up vote 1 down vote accepted

If they are in an alignment format already, the identities and mismatches are already calculated. So you have something like this:

Aln1: ACTGGTTGTCCAACCGTAATCGAAG

Aln2: ---GGTTGTCCAATTC---TCGAAG

Capture each one into a string, and simply enumerate over them. Something simple like this works:

mutations=0
for i,j in zip(aln1,aln2):
    if i != j and i != '-' and j != '-':
        mutations+=1

It depends on your personal criteria though, if you want to include gaps as mutations, etc.

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Where are i and j coming from? –  user1647556 Sep 26 '12 at 20:06
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try to read in FASTA file and store each sequence as string. You can certainly organize the sequences in a dictionary using text in the '<' line as key. If a gene is of the same length as a reference sequence without mutation, [i for i, a in enumerate(gene) if a != reference[i]] will return a list of position of mutations. its length will be the number of mutations. If mutation involves missing or added AA, it will be much more complicated.

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