Check if blastn gene matches are of entire genes or of parts of genes
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17 months ago
langziv ▴ 70

Hello,
I run blastn of specific bacterial genes against Klebsiella's plasmids' sequences.
I need to check if the matches are of entire gene sequences, in order to filter out partial gene matches.
The first thing I thought of was using blastx, but it's been a while since I last did such an analysis and I wish to check if there's a better recent approach. What do you think about blastx as the next step?
Another approach I thought of was comparing the query genes' lengths with the matches' lengths, but that way, in case of partial length matches, I don't know if the genes on the plasmids are functional or not.
Thanks.

blastx blastn bacteria • 1.6k views
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What exactly is your goal? Do you want to find genes in plasmid sequences that you sequenced? There are tools to do that (e.g. prokka)

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I'm looking for specific genes in all plasmids of a changing bacteria species. Now I'm working on Klebsiella.
Can such tools be used only for specific genes?

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You can run Prokka and get the full list of genes in the plasmid, then look for your gene of interest

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What do you think about using blastx?

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Can you clarify what type of sequence is in your query? Fasta/fastq/full length?

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Sure.
The queries are fasta files of specific genes.

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If you know where the genes are on your plasmids then you could use BLAT perhaps even minimap2 to look for end-to-end hits.

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What do you think about using blastx?

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Blastx cannot be used because it uses a protein database. You could use tblastx in case the sequences are very divergent. However, if you get good hits with blastn already then you probably don't need this.

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Please clarify if you know what plasmids you are working with and also know what genes they have. If you know this information then it would simplify things to a large extent.

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I know what plasmids I'm working with. I have their fasta and GenBank files.

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17 months ago
Asaf 10k

What you should want to do is predict open reading frames in the plasmid sequence and then compare them, with global alignment, to the gene or genes of interest. You would prefer this path since you want to check if the proteins encoded are the same, if you just run a local alignment tool like BLAST you might end up clipping the ends of the protein if the match is poor there.

The simplest way to do this (as it is done for more than 20 years) would be using tools from EMBOSS : getorf and needle. You can either install it locally or run on one of the publicly available servers like this.

More automated and up to date tools to consider are prokka that will give you the entire annotation of your plasmid, then you can just look for the gene of interest by homology group or sequence.

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