Filtering Fasta Sequences By Chromosomes Names From A Big Fasta File
5
7
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12.4 years ago
sthait ▴ 130

Hello,

I wish to filter from a big FASTA file only sequences related to chrs 1-22, X and Y. An example of FASTA sequence is:

>ENSG00000119314|ENST00000210227|PTBP3|9|-1|115024785
GGGTGGCAGGTGCCTGTAATCCCAGCTACTCCAGAGGCTGAGGCAGGGGAATTGCTTGAG
CCTGGGAGGCAGAGGTTGCAGTGAGCCGAGATTGTGCCACTGCACTCCAGCCTGGAGTCT
CACTTTGTCACACAGGGTGGAGTGCAGTGGTGTGATCTCGGCTCACTGCAACCTCTGCTT
ACCGGGTTGAGATTCTCCTGTCTCAACCTCCTGAGTAGCTGGGATTACAGGCGTGCACCA
CCAAGCCAGACTAATTTTCCTATTTTTAGTAGAGATGGGGGGTTTCACCATGTTGGCCAG...

>ENSG00000236011|ENST00000211377|GPANK1|HSCHR6_MHC_COX|-1|31616421
CCCTATTCCTACCTAACCTCCCCTCAGGACTCAGGCTCCAATGTGTTGAGCCCCAACTCC
TTCCCATAAGACTGCCACACGGTGCTTTCCTTTCCCTTCTTCAACACTCACCAATGGGAA
GCATTGGCTGGTTCTCACAGTACACACGAGGACAGTAACCAAAGTCTCCTTGCTGGTACT
TTTCCAACTGAGGTGAATACAATGGAAGGGGTTGGCAGGTAGATGTAAAGAAGAGGCAAC
TCCCTTCGCAGCCCAACCCATACCACTCTGTCCCCCACTCCTCCCACCTCTGTCCAGAGG
CCCCTTCTCTGGACTAGACGGGCTCTCAAACTTCTGTGTTGCCTTTCTTCCAATTAGGCA
GGCTACAAACCATCAGAGCCATTTGTTGTTTGTTCCTTGAGGAAGAGGCAGTCTATCACA
ACTCTCTGATTCAAGGTCTGTCTCCCTCCCTGAAAACAATCCCTTCAGGATGACCCCCAA...

>ENSG00000087494|ENST00000201015|PTHLH|12|-1|28115255
TCCGCTCACGGGCCCCGAGACCCCCGAAGTTCCCATGGAGCCTAAGATCCCCAGGAGCCA
AGCCTGCCCCGTCCCTGCGGATCAGCTTCCTAATGGGCGACCCAAGTCTATCGCAGGCGG
TGGGGATGAGGACGCTGGGTGGGAGGAGGGGAGGGGAGGCTGAAAAAGATCATCCCCCTT
GCCCTAAGGCCTCTCCCAAGACCCTGGACCCCTGCCCTAAGAGACTCAGGCCTCCCTTGC
TGCAGTGGGAGCGCAAACACCAGGGCAGGAGACTCCAGAGAAGGAGCGCATAACTCAACG
TTTGCTCTCCTGAAGCCTTATTTCTGATAAAAATTACAGAAAAGTTAGGCAGGATCCAAA
GACACCGTAATGACCAGCTCAAAGCCAAACAGACAGGACATCCAGTGCGGGTGTCTGGAT...

As you can see in the forth place after "|" there is the chromosome name: in the first one is: 9 the second one is: HSCHR6MHCCOX and the third one is: 12

I want to create a new FASTA file containing only 9, 12 sequences and in more generally 1-22, X and Y sequences.

What is fastest way to do it?

Thanks,

Tom.

fasta filter chromosome • 31k views
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24
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12.4 years ago
Leszek 4.2k

You can use samtools for that:

#index a genome
samtools faidx human_genome.fa
#select chromosomes or regions
samtools faidx human_genome.fa chr1 chr2:1:2000 [...] > human_selected.fa
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1
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I got the following error:

[faibuildcore] different line length in sequence 'ENSG00000006282|ENST00000006658|SPATA20|17|1|48624450'. Segmentation fault

what could be the problem?

thanks.

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0
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error is the result of wrong formatting of your fasta file... all sequence lines need to have the same max lenght, ie 60 or 70. anyway, you should index the genome, not your multifasta file.

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0
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just one quick observation, the correct way to write the segment of the chromosome is chr2:1-2000, not chr2:1:2000

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0
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THank you, leszek. It is the most convenient and comparatively fastest way I have found to remove the scaffolds in the reference genome.

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7
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12.4 years ago

You can do the following:

chr=$(seq 1 1 22)" X Y"
for i in $chr ; do 
    grep ">" input.fa | grep "|$i|" | awk 'BEGIN {FS=">"} {print $2}' > selection_$i
    samtools faidx input.fa `cat selection_$i` > output_$i.fa
done
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1
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It did not work for me - nothing was printed to file. However this modification did:

for i in $chr ; do
    samtools faidx $fasta $i  >> chr_sequences.fa
done

It should be noted that this puts all sequences into a single file.

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0
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What is $fasta here? You did not make this clear...

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0
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$fasta is a variable that represents the input fasta. It should be defined before the loop as fasta=my_fancy.fasta

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thanks, i'm pretty new in this. the code you gave me - in which program should I run it - terminal/perl/python?

tom.

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0
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This is a bash script, so you can just run it as is in a terminal.

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0
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12.4 years ago
JC 13k

if you want Ensemble gene models, you can use BioMart to obtain your sequence filtered: http://uswest.ensembl.org/biomart/martview

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0
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9.5 years ago

You can do some pattern matching using pyfaidx:

faidx --regex "^.+\|.+\|.+\|[[1-9][0-2]?|[XY]]" input.fa > output.fa
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