This is somewhat of a follow-up from previous posts (most recently C: How to determine which NCBI sequence to map against (multiple sequences for sing ). I was recently given a paired-end .fastq files (where each read has about 150 bases). The wet-lab researchers believe it is from an isolated strain of bacteria likely Helicobacter (this may be questionable). It was taken from dolphin stomach.

My job is to determine the identity (closest species etc.) of these samples. I have been attempting this for weeks and am stuck. Below are a few approaches I have tried:

1. I created contigs using SPAdes. I blasted a few of the contigs. Some seemed to align to Helicobacter cetorum MIT 00-7128. So, I downloaded that as a reference and aligned the sample to it using BWA. It had only 13% mapping rate. I also noticed that some contigs (shorter ones) blasted to Mus musculus/ Homo sapiens.

   I thought I should do a more sophisticated approach than blasting contigs. So, I tried (2), (3), (4) below:

2. Downloaded all “Complete genomes” of “Helicobacter” genus from NCBI (n=221). Used sourmash to compute k-mer sequences to determine relatedness of genomes. The highest similarity was 43.5% to Helicobacter pylori P12, but there were dozens of similarities with almost the same percentage to other Helicobacter strains.

3. Ran Kraken on Galaxy against a database of "plasmids", "viruses", and "bacteria". It had only 14% bacteria classified (and even less virus/plasmid), with most (5.66%) mapping to Helicobacter pylori.

4. Ran sendsketch on the contigs. It had WKID = 38.9%; KID = 0.05%; ANI = 96.6%; Contam = 2.5% for H. macacae (and similar numbers for H. mastomyrinus) and WKID = 1.1%; KID = 0.85%; ANI = 84.8%; Contam = 1.7% for H. cetorum MIT 00-7128.

   I thought the numbers above seemed low (please let me know if you think otherwise). They also do not seem consistent (with H. pylori showing up more in sourmash and Kraken and H. macacae showing up most in sendsketch) - but still that probably does not matter given how low these values are anyway.

5. In my latest post (linked above), a user suggested taking small selections of reads (~20-25) and blasting. I did this for both the first 25 bases and the last 25 bases in the file. BlastN on the first 25 bases had Helicobacter cetorum MIT 00-7128 with lowest e-value (3e-39), megablast on the first 25 bases had "no significant similarity found message", BlastN on the last 25 bases had Helicobacter felis ATCC 49179 with lowest e-value (1e-25), and megablast on the last 25 bases had Helicobacter felis ATCC 49179 with lowest e-value (3e-19). I am not sure if there are certain parameters I should use (such as blastN versus megablast) and whether theses results seem consistent - especially because the highest WKID value from sendsketch was a different Helicobacter species.

I do not have much experience at all with this type of analysis. Over the weeks, I feel like I am working in circles and throwing different software at this sample. My main findings so far: 1) There may be contamination, 2) Mapping/alignment/similarity scores seem low, 3) Different software can point (despite being low in value) to different Helicobacter species.

The biologists press me to tell them what species their sample is and I have been unable to feel confident about giving an answer. My worries are that it could be that it is not bacteria (maybe archaea), is too contaminated, is not "isolated", etc.

For anyone with experience, what would you recommend to someone in my position to confidently determine what species this is (if that even seems possible at this point)? Specifically:

1. How should I determine if contamination should be removed and how should I do so safely (if needed)?

2. When does one feel confident they can report the species back to biologists? Are my numbers above indeed too low and conflicting?

3. How can I determine this is isolated bacteria? And not something else like archaea or pure contamination or multiple species?

4. What other approaches should I take to determine the species (especially interested to hear ideas that add something new to what I have already tried, i.e. are not simply throwing another software similar to the ones above at it) :oD .

I apologize for the long post (wanted to be clear about what I have tried). Thank you for sharing your ideas.

I will only address a few things since there is so much to unpack.

It was taken from dolphin stomach.

Since we are starting there, there is no way to know what may have been in there to begin with. Idea that there would be only one species and that one would be able to identify it with certainty is very naive.

Some seemed to align to Helicobacter cetorum MIT 00-7128. So, I downloaded that as a reference and aligned the sample to it using BWA. It had only 13% mapping rate.

It is possible that there is some H. cetorum in this sample (13% if you want to go with your number). And then there could be tens of other things. It is also not surprising that you find Helicobacter spp. as prominent member. It is consistent with human stomach microbiome, which shows a similar trend (see paper linked below).

I also noticed that some contigs (shorter ones) blasted to Mus musculus/ Homo sapiens.

This could simply be contamination since a dolphin is unlikely to have those in their stomachs. It is possible that you may have some dolphin DNA that was in your sample (eukaryotic DNA) that is similar to human/mouse.

I did this for both the first 25 bases and the last 25 bases in the file.

I was the one who had suggested that. I hope that actually means 25 reads and not bases. If you took 25 bases from each read then please go back and re-do the blast analysis.

The biologists press me to tell them what species their sample is and I have been unable to feel confident about giving an answer.

Bottom line is this sample is unlikely to contain only one bacterial species since it was collected from an environment which could harbor many different bacteria. See this example paper for human gut microbiome. There is also a review on human stomach microbiome which finds more than one genera.

Also remember that you could be looking at data from species of bacteria/archaea that have never been seen before (dolphin stomach is pretty exotic habitat) so there may be no absolute identification possible at species level (unless they sample more dolphin stomach contents and you find similar sequences there).

You should perhaps do metagenomic data analysis to get an overall picture of what is in your data.

I created contigs using SPAdes. I blasted a few of the contigs. Some seemed to align to Helicobacter cetorum MIT 00-7128. So, I downloaded that as a reference and aligned the sample to it using BWA. It had only 13% mapping rate. I also noticed that some contigs (shorter ones) blasted to Mus musculus/ Homo sapiens.

"aligned the sample" meaning you mapped the PE reads to the reference?

How should I determine if contamination should be removed and how should I do so safely (if needed)?

If you want to be really sure about contamination, if they sequenced negative controls you could compare kmer overlap of your negative controls to your samples.

When does one feel confident they can report the species back to biologists? Are my numbers above indeed too low and conflicting?

Do they want a microbiologist-style "is bug X here or not" / "which Genus X did you find" or a description of the stomach microbiome? If they have an a priori hypothesis they wish to test, you could report that after mapping reads to that reference genome that you didn't get complete overlap, which could be a overlap issue or a different species of same genus.

If the hypothesis is "which genus may be in my sample", using your kraken2 .report it should give some percentages for given samples (note that there is mini kraken, standard kraken and maxikraken databases floating about, which will affect results). Digging through your kraken .out it'll give the C/U (classified/unclassified), taxonomy, nt, and the kmer composition. You can check the output for all the Helicobacters you're interested in and check out how many kmers in a contig were used to call it, which can be a useful confidence measure. If a contig is say 0:100 Helicobacter_number_here:1, then 100 kmers were unclassified and it called it based on 1 kmer, which might not be as exciting as something with a high number of kmers.

How can I determine this is isolated bacteria? And not something else like archaea or pure contamination or multiple species?

Multiple related species might be a tricky one to parse out with WGS alone. If the assembly graph is tangly it'll complicate things. Confidence in species calls might increase if the wetlab folks attempted to culture (selective/differential), then isolate, grow up and sequence, versus MAGs derived from a metagenome. Your kraken report should give some insights into community composition. Running metaphlan2 on the paired end reads may give a different picture.

Another option for contamination is something like VizBin, which will let you bin things out by hand. It's a bit more...manual...than I'd like, but for a reasonably uncomplicated sample like stomach it may be helpful. You can "gate" (to borrow the term from flow cytometry) contigs in a 2d tSNE grid, export them, and then figure out their taxonomies and the like. And if all your helicobacters are clustered together in the same blob, you can seperate them visually from the rest of the sample and carry out your annotation that way. If you downselect too soon (eg, only the reads/contigs that map to a given Helicobacter) you might be throwing too much out too soon.

What other approaches should I take to determine the species (especially interested to hear ideas that add something new to what I have already tried, i.e. are not simply throwing another software similar to the ones above at it) :oD .

While you're at it, running any of the metagenome binning pipelines may be useful. Bin integrity could be checked with checkm, et al. Then individual bins assessed for function/genome architecture/taxonomy. an'vio is a pretty useful turnkey program to do most of these functions, and I'm retooling towards using an'vio myself.

An additional resource to the segata paper is https://astrobiomike.github.io/genomics/ .

Here is an idea that hasn't been mentioned yet: try to find small ribosomal subunit rRNAs in your sample. That can be done with SSU-ALIGN, RNAmmer or Barrnap. Assuming you identified some 16S/18S rRNA sequences, their placement within a larger SSU trees of prokaryotes and eukaryotes should give you a good idea about what is present in your sample.

Separately, you did a good job with what you have tried so far. I would say that your results do indicate the presence of Helicobacter-like microbe, but it is tough to say how prevalent it is.

As @MensurDlakic suggested, finding rRNA genes would be key. One easy way to do this would be to use phyloFlash on your library reads (works even with raw reads; link for the tool here: https://hrgv.github.io/phyloFlash/). Also, take a look into the GC-coverage plots of your assembly with each blob on your plot being taxonomically annotated using the NCBI nt database. You can conveniently generate such a plot by using gbtools (manual here: https://github.com/kbseah/genome-bin-tools/wiki/0.-Introduction). If there are contigs representing eukaryotes in your assembly, they will appear at the bottom end (meaning low coverage) of your GC-coverage plot; bacteria will be represented by higher coverage contigs that may (or may not) also differ in their GC-contents. If there are multiple bacterial taxa detected, they will appear as differentially colored blobs with a distinct taxonomy, GC- and coverage-spread on the plot. Using barrnap along with gbtools, you can additionally see on the plot the SSU rRNA harboring contigs (along with their taxonomic affiliation). I tend to not that heavily rely on read-level metagenomic classifiers such as Kraken2 or metaphlan2 (their results need to be always taken with a pinch of salt!). As a final step, I would run CheckM on your assembly to estimate completeness/contamination. Hope this helps!