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I need to remove some base pairs from a fasta file. This is the example of my input file

>\>NODE_1
GTTGGCCGAGCCCCAGGACGCGTGGTTGTTGAACCAGATCAGGTCCGGGCTCCACTGCAC
GTAGTCCTCGTTGGACAGCAGCGGGGCGTACGAGGCCAGCTTGACCACGTCGGCGTTGCG
CTCGAGGCCGGTCATGAACGCGGCCTCGGCGAGGGCGTTCTTCCAGGCGTTGCCCT  
\>NODE_2 
GTTGGCCGAGCCCCAGGACGCGTGGTTGTTGAACCAGATCAGGTCCGGGCTCCACTGCAC
GTAGTCCTCGTTGGACAGCAGCGGGGCGTACGAGGCCAGCTTGACCACGTCGGCGTTGCG
CTCGAGGCCGGTCATGAACGCGGCCTCGGCGA

and i have 20 these kinds of nodes in my file. My aim is to shorten the file like this

>\>NODE_1
GTTGGCCGAGCCCCAGGACGCGTGGTTGTTGAACCAGATCAGGTCCGGGCTCCACTGCAC
GTAGTCCTCGTTGGACAGCAGCGGGGCGT  
\>NODE_2 
GTTGGCCGAGCCCCAGGACGCGTGGTTGTTGAACCAGATCAGGTCCGGGCTCCACTGCAC
GTAGTCCTCGTTGGACAGC

Right now, I am just able to read the files in R.

x<-readLines("input file.fa", n = -1L, ok = TRUE, warn = TRUE)

Can you guide me how can i proceed this?

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What does it mean to remove base pairs? I have not studied genetics... –  Petar Minchev Aug 1 '11 at 10:07
    
For people with no biology background, I think you should clarify what a base-pair is (eg. how you are shortening your node by removing it). –  Nico Huysamen Aug 1 '11 at 10:09
    
I've added a link so long, but please clarify the question to make it easier for people to help. –  Nico Huysamen Aug 1 '11 at 10:11
1  
JProfiler, LOL:) –  Petar Minchev Aug 1 '11 at 10:13
1  
Updated link to wiki. I don't see the sequence shortening logic in your example, the 1st 60bp are constant, why are the next sequences shortened? they are not complimentary in any dimension .. –  Alex K. Aug 1 '11 at 10:17

1 Answer 1

For a base-R solution, use substr. Yet the better idea is to use Bioconductor's Biostrings' functions, i.e.

readFASTA("input.fa")->x
shortX<-subseq(x,start=1,width=100)
writeFASTA(shortX,"output.fa")
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