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**maubp** · 11-22-2013, 02:50 PM

Normally you'd assign GO terms to genes/proteins (typically short), not entire genome contigs (typically long).

You should look at gene finding, and perhaps automated annotation in general.

**Hel** · 12-10-2013, 03:50 AM

Hi NGS_New_User,

I also have the same question. I have a de novo assembled transcriptome to analyze in gene ontology terms. Please maubp, could you explain how to get genes/proteins from our data? Because I only have contigs (and unassembled reads)..

Thanks in advance!

**rhinoceros** · 12-10-2013, 04:08 AM

Originally posted by Hel View Post

Hi NGS_New_User,

I also have the same question. I have a de novo assembled transcriptome to analyze in gene ontology terms. Please maubp, could you explain how to get genes/proteins from our data? Because I only have contigs (and unassembled reads)..

Thank in advance!

Why not:

1. Predict proteins
2. Blastp against nr (tabular output)
3. Map to GO with this file
4. Sort for best hits with a GO match

**sphil** · 12-10-2013, 05:32 AM

Originally posted by rhinoceros View Post

Why not:

1. Predict proteins
2. Blastp against nr (tabular output)

or
2. Blastp against nr (XML output)
3. load into Blast2GO
4. do you analysis...

prediction of proteins you can go with augustus but there are several other programs which are capable.

**mcnelson.phd** · 12-10-2013, 05:44 AM

Originally posted by Hel View Post

Hi NGS_New_User,

I also have the same question. I have a de novo assembled transcriptome to analyze in gene ontology terms. Please maubp, could you explain how to get genes/proteins from our data? Because I only have contigs (and unassembled reads)..

Thanks in advance!

You'll need to get the nucleotide sequence of all possible ORFs that are found in your contigs. To do that you can use Glimmer, GeneMark, or a few other ORF callers although the first two are probably the most popular. Then you can get a multi-fasta of all the ORFs and run those through blast2GO.

**Hel** · 12-11-2013, 07:28 AM

Thanks to all

. I'm sorry but I don´t understand everything.

rhinoceros) Which tool to predict proteins?

sphill) Well, Blast2GO already do the blast step, isn't it?

mcnelson.phd) My contigs came from RNA-seq, so all my sequences have been expressed. Do you mean that I have to select the portion of the contigs that is expressed? This confuses me.

Thanks in advance!

**maubp** · 12-11-2013, 07:34 AM

Originally posted by Hel View Post

sphill) Well, Blast2GO already do the blast step, isn't it?

Doing the BLAST online at the NCBI from within the Blast2GO tool is very slow. It is much faster to run the BLAST locally on a cluster, and import the BLAST results into Blast2GO for the annotation mapping step.

**sphil** · 12-12-2013, 05:47 AM

Originally posted by maubp View Post

Doing the BLAST online at he NCBI from within the Blast2GO tool is very slow. It is much faster to run the BLAST locally on a cluster, and import the BLAST results into Blast2GO for the annotation mapping step.

Yep that is exactly why i should go with local blast and then blast2go.

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