Hello,
In an old experiment dating back to 2014, some 16S libraries from plant samples were prepared, with the aim to identify the microbial community living/contaminating the surface of the fruits.
The primer choice was the couple 27F and 533R.
Sadly, once analyzed with QIIME2 and clustered, out of 12 samples, 10 had chloroplast DNA contaminations percentages up to 99% (80-99%), making them completely useless.
I'd like to run the experiment again, with Illumina technology, addressing the problem of the primers not being specific enough to distinguish between plastid and bacteria DNA.
At the moment, the only scientific paper directly addressing the issue I was able to find was this one, but it's quite an old one.
Any suggestions here? Thanks in advance.
Just to confirm, you want to resequencing the sample specimens but with illumina 16S sequencing and you want to know of a way to differentiate between bacterial and chloroplast 16S?
QIIME2 has a filter module you should checkout: https://docs.qiime2.org/2018.11/tutorials/filtering/
You can also filter with phyloseq https://joey711.github.io/phyloseq/
It might be possible to align all illumina reads to chloroplast 16S, then use any reads that don't align in downstream analysis.
Thanks for the suggestion, but I wasn't referring to this. I have already tried the qiime taxa filter-table function and it works like wonder, but it just removes the reads I'm not interested on from the QIIME 2tables.
The problem isn't about filtering data, but about obtaining data with a lower contamination rate since the very beginning. So my issue is about primers choice.
Right, apologies I misunderstood. Hopefully someone can provide some help.