how to merge many .fa files to one single target file containing list of amino acids #311
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when you want to assemble each gene in a single fasta file you want you use
the -Q rather -q to specify the query file. the capital Q tells atram to
assemble each one sequentially.
Is that what you did initially?
…On Sat, May 14, 2022 at 8:39 AM Upasana1991 ***@***.***> wrote:
Hi I am Upasana
I have 200 genome of anopheles sequenced at 30X
I have a list of single copy orthologs that I have generated using
proteomes of two reference genomes in Orthofinder. This gave me around 8322
single copy orthologs (list of amino acid sequence (.fa) files)
I went through the tutorial of aTRAM and was clear to me how each step was
written.
In the example you have used only one .pep.fasta file ; When I used one
amino acid sequence as. Target file, it worked, however
When I concatenated all the .fa files into one sinlge .fasta file
containing 11548 a.a sequences and used this as target file it didn’t work.
Is there a way I can use the list of .fa file from orthofinder results as
is?
Is there a correct way of putting all the .fa files into one fast file ? I
used this command “cat *.fa > TargetSCO.fasta”
Thanks for your time and help
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Yes thank you .
From: juliema ***@***.***>
Date: Monday, 16 May 2022 at 18:07
To: juliema/aTRAM ***@***.***>
Cc: Upasana Singh ***@***.***>, Author ***@***.***>
Subject: Re: [juliema/aTRAM] how to merge many .fa files to one single target file containing list of amino acids (Issue #311)
when you want to assemble each gene in a single fasta file you want you use
the -Q rather -q to specify the query file. the capital Q tells atram to
assemble each one sequentially.
Is that what you did initially?
On Sat, May 14, 2022 at 8:39 AM Upasana1991 ***@***.***> wrote:
Hi I am Upasana
I have 200 genome of anopheles sequenced at 30X
I have a list of single copy orthologs that I have generated using
proteomes of two reference genomes in Orthofinder. This gave me around 8322
single copy orthologs (list of amino acid sequence (.fa) files)
I went through the tutorial of aTRAM and was clear to me how each step was
written.
In the example you have used only one .pep.fasta file ; When I used one
amino acid sequence as. Target file, it worked, however
When I concatenated all the .fa files into one sinlge .fasta file
containing 11548 a.a sequences and used this as target file it didn’t work.
Is there a way I can use the list of .fa file from orthofinder results as
is?
Is there a correct way of putting all the .fa files into one fast file ? I
used this command “cat *.fa > TargetSCO.fasta”
Thanks for your time and help
—
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<#311>, or unsubscribe
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Hi I am Upasana
I have 200 genome of anopheles sequenced at 30X
I have a list of single copy orthologs that I have generated using proteomes of two reference genomes in Orthofinder. This gave me around 8322 single copy orthologs (list of amino acid sequence (.fa) files)
I went through the tutorial of aTRAM and was clear to me how each step was written.
In the example you have used only one .pep.fasta file ; When I used one amino acid sequence as. Target file, it worked, however
When I concatenated all the .fa files into one sinlge .fasta file containing 11548 a.a sequences and used this as target file it didn’t work.
Is there a way I can use the list of .fa file from orthofinder results as is?
Is there a correct way of putting all the .fa files into one fast file ? I used this command “cat *.fa > TargetSCO.fasta”
Thanks for your time and help
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