16S rRNA merge forward and reverse primers
2
0
Entering edit mode
3.4 years ago
ddowlin ▴ 70

Hi all,

I have received 16S rRNA sequencing data for ~ 100 samples.

I want to use these sequences to identify the samples to genus level using the NCBI BLAST 16s bacteria and archaea database.

For each sample I have a forward primer fasta sequence (7F) and a reverse primer fasta sequence (1540R).

For ~40 I have a 'spliced' sequence which contains a fasta with a merged forward and reverse primer data. This was provided by the sequencing company. ~60 samples do not have a 'spliced' sequence.

My questions are:

1.) Is there a best practice protocol for merging forward and reverse primers?

2.) Can I concatenate the forward and reverse primer sequences into a single fasta file and search using these, or will this introduce biases?

3.) For the sequences that were not spliced, should I favour one of the two primers for identification purposes?

Many thanks!

d

16S taxonomy rRNA microbiology primers • 2.1k views
ADD COMMENT
0
Entering edit mode

For each sample I have a forward primer fasta sequence (7F) and a reverse primer fasta sequence (1540R).

Is this a Sanger sequencing from a 16S rRNA clone library?

ADD REPLY
0
Entering edit mode

No, this was Illumina sequencing.

ADD REPLY
1
Entering edit mode
3.4 years ago
Mensur Dlakic ★ 28k

I am not sure that I understand everything you have done, so take my answers with a grain of salt. For example, are these pure culture or metagenomic samples?

1.) Is there a best practice protocol for merging forward and reverse primers?

I think you mean here merging results of forward and reverse amplicons (sequencing results). They need to have a significant overlap in order to be merged. Ordinarily it would be enough to have an overlap of maybe 20-40 bases, but 16S sequences are very similar even between different species. That's why you may need longer overlap than that - I would ask the company how they did it.

2.) Can I concatenate the forward and reverse primer sequences into a single fasta file and search using these, or will this introduce biases?

Only if you are absolutely certain that you have sequenced a pure culture sample, and if you know that your species has a single 16S rRNA. In such a case using a concatenated sequence may give you a cleaner result, but don't forget to reverse-transcribe one of them so you have the same strand.

3.) For the sequences that were not spliced, should I favour one of the two primers for identification purposes?

See above about the pure culture. Either way, I think both sequences will provide some information.

ADD COMMENT
1
Entering edit mode
3.4 years ago
noodle ▴ 590

I want to use these sequences to identify the samples to genus level using the NCBI BLAST 16s bacteria and archaea database.

Release the kraken!

ADD COMMENT

Login before adding your answer.

Traffic: 2357 users visited in the last hour
Help About
FAQ
Access RSS
API
Stats

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by the version 2.3.6