Hello,

I've seen similar issues with my own data, and in general I think that taxonomic profiles should always be taken with a pinch of salt. Off the top of my head, a few possibilities:

1. Metagenome read profiling methods can be quite sensitive to the database used and the cutoffs for assigning a given read to a taxon. It might be worth trying a different pipeline like Kraken (https://www.ncbi.nlm.nih.gov/pubmed/24580807) to see if you get similar results.

2. rRNA operon copy number can vary between different microbial species. E.g. if species A has two copies of the 16S gene per genome, and species B has only one, one, then A might appear to be twice as abundant as B. You could try profiling only the 16S sequences from the metagenomic shotgun libraries to see if this gives a better fit to your amplicon libraries, e.g. with Emirge (https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3219967/) or Matam (https://www.ncbi.nlm.nih.gov/pubmed/29040406). My colleagues and I are working on a pipeline for quick screening and comparison of metagenome libraries for SSU using Emirge and other tools (https://github.com/HRGV/phyloFlash).

3. Amplicon libraries can be quite heavily influenced by amplification and primer biases during PCR (e.g. see https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3592464/)

Hope this helps!

-- Brandon

Hi,
Thanks so much for the reply. These make sense to me. And now I am totally agreed. During these days after I posted the thread, I have been trying many different method and software. I found just taxonomic profiling cannot be accurate, and the different result got from the comparison between 16S amplicon is expectable.
Kraken gives me 2% reads hit NCBI. It is lucky to meet PhyloFALSH, which can be used for extract 16S reads and give me the taxonomy result. 0.107% reads hits to SILVA database. Still waiting for the publication of PhyloFLASH.
I have also tried a software- Kaiju, which got 47% reads hits to NCBI nr database, 31% reads hits in RefSeq Complete Genomes database, 38% reads hits in proGenomes database.
Interesting, challenging but confusing. Maybe for environmental samples, assemble is necessary.
Looking forward to more suggestions shared from you.
Best.