I have been reading around the analysis of metagenome recently and came across methods of annotation that use raw reads or just assembled metagenomic sequences. Does it bias the annotation to not assemble and bin the metagenome into MAGs or is it safe to assume you will not get any "hybrid" gene where half come from one theoretical MAG and half from another when annotating raw reads?

Apologies if this is a silly question, i am not to familiar with how annotators work.

Hi,

I guess the difference relies on the confidence of the annotation. Annotating raw reads (I guess you mean short-reads, raw somehow suggests the reads were not trimmed in quality and for adapters - and they should be) is more difficult as you can easily understand due to its length (~150 bp) than annotating assembled contigs or scaffolds from MAG (>1Kb). Particularly it would be impossible to try to annotate the taxonomic origin of those reads, with the exception of taxonomic markers such as ribosomal RNA genes/reads, although you can annotate them functionally with some success using interproscan against InterPro database of protein domains and protein families, because these rely on short conserved regions. This approach was actually applied by previous EBI metagenomics pipeline (available online at: https://www.ebi.ac.uk/metagenomics/pipelines/4.1). Although someone could argue that this was chosen due to computational limitations of an online service provider. Actually, the most recent version performs assembly (at: https://www.ebi.ac.uk/metagenomics/pipelines/5).

Therefore, if you want to annotate your metagenomes at taxonomic and functional levels as best as possible, i.e., get better annotations of genes and taxa, I would say that you need to try to assemble your metagenomes.

I hope this helps,

António