Measure particulates in growth medium
Certain growth media have unexpectedly high particle concentrations. This can lead to confusing results, particularly during the lag phase when bacterial concentration is still low. Step-by-step instructions are given below for how to measure the concentration objects in the growth medium.
Step by step
Use a serological pipette to collect a small sample of the cultivation medium.
Vortex 30 seconds at max speed to ensure an even distribution of particles
Dilute 1:100 in diluent
Add 101 µL of sample to 10 mL of diluent.
Vortex 10 sec., max speed.
Transfer the tubing kit to the diluted sample.
Click Measure .
Do you get the error conductivity too high?
Some cultivation media have very high conductivity and a 1:100 dilution in standard diluent is not sufficient to bring the diluted sample within the accepted conductivity limits.
You can typically solve this issue by using a 1:201 dilution: Simply add 50 µL of sample to 10 mL of diluent. For more information, please see the section Hit the right concentration.
Results and implications
We focus on the cells/mL concentration as it may artificially increase the perceived cell count. The total/mL value is also important, but mainly because higher dilution might be necessary if there's notable particulate contribution from a specific source.
If the 1:100 dilution is below 30,000 cells/mL, background particulate contribution is negligible.
If the 1:100 dilution exceeds 30,000 cells/mL, choose one of the mitigation strategies.
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