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WeigelWorld Opentron2 duct-tape
These duct-tape scripts go between tecanalyze and the opentron protocol language itself.
Installation
tl;dr:
python3 -m pip install weigel-ot2tools
To use these tools (CLI only for now), first install with python3 -m pip install weigel-ot2tools. If you know what pipx is, use that. If pip install
fails on your laptop, you can do this on a linux server as these tools need
no GUI. If that fails, email me.
Then, use either ot2ools variable_stock or ot2ools constant_stock to
generate the ot2 scripts.
Manual
There are two main ways of doing dilutions: constant-stock and variable-stock.
Constant stock only pipettes water into plates with the opentron, after which we use the viaflow to transfer across a constant volume of stock DNA/RNA. This is faster, easier, and better if you have labile stocks like RNA you don't want hanging around in the opentron for hours. However, it has limited dynamic range (i.e. can only do up to 20-fold dilutions), and produces highly varying amounts of diluted DNA/RNA.
Variable stock has the opposite properties: by pipetting variable amounts of both stock and diluent, we can have much greater dilution ratios (up to 200x), and we can (but don't have to) produce a constant volume of diluted DNA/RNA. However, it's slower (max 3 plates at a time), and you need to have your stock open to the world and at room temp for much longer, so can cause problems with particularly sensitive things like dirty RNA extractions.
ot2ools constant_stock
This is the "normal" Pathocom way to do dilutions. We use the opentron only to
pipette a varying amount of water, then use the viaflow 96 head to transfer
a constant amount of stock across. This can be used with the files directly out
of tecanalyze. You need only columns
plate_name, well, conc (these can be called something else and there can
be extra columns in the file, see the CLI --help output).
ot2tools constant_stock \
--protocol-script-dir protocols/ \
--conc 5 \
--volume 10 \
--pc plate_name --wc well \
--cc conc \
quantifications.csv
ot2ools variable_stock
First, prepare a csv or tsv with at least the following columns: plate, well,
stock_volume, water_volume. The column names can vary, you just need to give
the actual names with --plate-column etc. You'll get an error if there's
a mismatch.
ot2tools variable_stock \
--protocol-script-dir protocols/ \
--pc Plate_name --wc Well \
--hc Water --sc DNA quantification.csv
Full help follows
$ ot2ools variable-stock --help
usage: ot2ools [-h] [-o PROTOCOL_SCRIPT_DIR] [-p {p10,p50}] [-m MIN_VOLUME] [-M MAX_VOLUME] [--pc PLATE_COLUMN] [--wc WELL_COLUMN] [--hc WATER_COLUMN] [--sc STOCK_COLUMN] instructions
positional arguments:
instructions Instructions file csv
options:
-h, --help show this help message and exit
-o PROTOCOL_SCRIPT_DIR, --protocol-script-dir PROTOCOL_SCRIPT_DIR
Output dir
-p {p10,p50}, --stock-pipette {p10,p50}
Which pipette to use for stock pipetting
-m MIN_VOLUME, --min-volume MIN_VOLUME
Minimum volume to transfer
-M MAX_VOLUME, --max-volume MAX_VOLUME
Maximum volume of destination well (combination of water+stock)
--pc PLATE_COLUMN, --plate-column PLATE_COLUMN
Column name for plate
--wc WELL_COLUMN, --well-column WELL_COLUMN
Column name for well
--hc WATER_COLUMN, --water-column WATER_COLUMN
Column name for water volume
--sc STOCK_COLUMN, --stock-column STOCK_COLUMN
Column name for stock volume
ot2ools pool_by_volume
This script is for pooling a plate of libraries according to their concentrations. This needs a csv with the following columns: plate, well, volume, pool. Like above, these names can be changed with CLI arguments. This requires that you've already calculated how much volume you need from each sample. The labware layout is a 24-well rack of eppies, with up to 5 plates of source libraries and 5 boxes of tips to be pooled into up to 24 pools.
PLEASE NOTE: your quantifications need to be reasonably accurate, and need to be taken after individual SPRI cleanup for this to be accurate. If you just do picogreen on the post-PCR libraries, the amount of library is often much less than the amount of dimer, defeating the entire purpose of this pooling. If need be, use a larger volume of DNA (e.g. 3uL) for quantification of low-concentration libraries.
$ ot2ools pool-to-eppies --help
usage: ot2ools [-h] [-o PROTOCOL_SCRIPT_DIR] [-p {p10,p50}] [-m MIN_VOLUME] [-M MAX_VOLUME] [--pc PLATE_COLUMN] [--wc WELL_COLUMN] [--vc VOLUME_COLUMN] [--lc POOL_COLUMN] instructions
positional arguments:
instructions Instructions file csv
options:
-h, --help show this help message and exit
-o PROTOCOL_SCRIPT_DIR, --protocol-script-dir PROTOCOL_SCRIPT_DIR
Output dir
-p {p10,p50}, --stock-pipette {p10,p50}
Which pipette to use for stock pipetting
-m MIN_VOLUME, --min-volume MIN_VOLUME
Minimum volume to transfer
-M MAX_VOLUME, --max-volume MAX_VOLUME
Maximum volume of destination well (combination of water+stock)
--pc PLATE_COLUMN, --plate-column PLATE_COLUMN
Column name for plate
--wc WELL_COLUMN, --well-column WELL_COLUMN
Column name for well
--vc VOLUME_COLUMN, --volume-column VOLUME_COLUMN
Column name for water volume
--lc POOL_COLUMN, --pool-column POOL_COLUMN
Column name for stock volume
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