A PrIMEr infereNce TOolkit to facilitate large-scale calling of metabarcoding amplicon sequence variants.
PIMENTO’s employs a dual primer inference strategy, which are:
- Standard primer search: based on fuzzy regex search queries to a library of curated standard primer sequences.
- Primer cutoff prediction: based on the identification of the primer cutoff point from analysis of patterns of base-conservation at the beginning (and end, for single-end libraries) of reads. Consensus sequences are then generated as inferred primers using the predicted cutoff.
PIMENTO also implements an "are there primers?" function to predict the presence of primers in sequencing reads in case no standard primer was found. This method is helpful in cases where it isn't known whether primer sequences are still present in the reads, and checking manually would not be trivial, i.e. for large-scale analysis pipelines.
PIMENTO is available on PyPi. To install it from PyPi with pip just run:
pip install mi-pimento
PIMENTO is also available on bioconda and can be installed like this with conda/mamba:
conda install -c bioconda mi-pimento
You can run either PIMENTO strategy with a single command. The tool will look for primers on either end, so both strategies will work on paired-end, single-end, or merged paired-end sequencing reads (though you would have to run it twice unmerged paired-end sequencing reads, one for each end).
pimento --help
Usage: pimento [OPTIONS] COMMAND [ARGS]...
Options:
--version Show the version and exit.
--help Show this message and exit.
Commands:
are_there_primers Predict whether primers are present in the input reads
auto Perform the primer cutoff strategy for primer
inference
choose_primer_cutoff Choose the optimal primer cutoff point.
find_cutoffs Find potential cutoffs using a BCV output.
gen_bcv Generate the base-conservation vector(s) (BCV)
std Perform the standard primer strategy for primer
inference
To run the standard primer strategy:
pimento std -i <fastq/fastq.gz> -p <primers_dir> -o <output_prefix> --merged-i <fastq/fastq.gz>: the input FASTQ reads file.
-p <primers_dir>: the path to the standard primers library to be used, with the default being PIMENTO's library. You can use your own library, or extend PIMENTO's. If using a different library than the default, make sure the primer FASTA files have this format:
>341F
CCTACGGGNGGCWGCAG
>338F
ACTCCTACGGGAGGCAGCA
>805R
GACTACHVGGGTATCTAATCC
>785R
CTACCAGGGTATCTAATCC
Where forward strand primers have the character F as the final character, and vice versa R for reverse strand primers.
-o <output_prefix>: the prefix to be used on output files.
--merged: this optional flag should be used when dealing with either merged paired-end reads, or single-end reads, so that PIMENTO can correctly identify reverse-orientation primers
<output_prefix>_std_primers.fasta: FASTA file containing the best found single or pairs of primers. Empty if none were found.
<output_prefix>_std_primer_out.txt: Text file containing the read proportions of the best found primers.
all_standard_primer_proportions.txt: Text file logging all the read proportions for every single searched primer.
To run the primer cutoff strategy:
pimento auto -i <fastq/fastq.gz> -st [FR/F/R] -o <output_prefix>NB: Running pimento auto executes the three subcommands generate_bcv, find_cutoffs, choose_primer_cutoff sequentially. You can therefore run each step of this workflow individually if you wish.
-i <fastq/fastq.gz>: the input FASTQ reads file.
-st [FR/F/R]: the selection of strands to perform primer inference for - F for forward, R for reverse, FR for both.
-o <output_prefix>: the prefix to be used on output files.
<output_prefix>_auto_primers.fasta: FASTA file containing the inferred primer sequences using the predicted optimal cutoffs.
To run the "are there primers?" utility:
pimento are_there_primers -i <fastq/fastq.gz> -o <output_prefix>-i <fastq/fastq.gz>: the input FASTQ reads file.
-o <output_prefix>: the prefix to be used on output files.
<output_prefix>_general_primer_out.txt: Text file containing a 1 or 0 depending on if a primer was found on the forward strand (first line) and the reverse strand (second line).
If you use PIMENTO in your work, please cite the Biorxiv pre-print:
PIMENTO: A PrIMEr infereNce TOolkit to facilitate large-scale calling of amplicon sequence variants
Christian Atallah, Lorna Richardson, Martin Beracochea, Robert D. Finn
bioRxiv 2025.07.04.663168; doi: https://doi.org/10.1101/2025.07.04.663168