3.3
Sampling and
Analysis
Prior to induction, samples after batch are taken to determine
viable biomass growth and potential metabolite accumulation. An
additional sample after the continuous adaptation phase must be
taken to again determine viable biomass and metabolite accumula-
tion. Sampling frequency during induction is highly dependent on:
l
The doubling time of the host organism.
l
Expected deviations in productivity.
For E. coli BL21 (DE3), samples are taken once to twice a day.
In addition to previously stated analysis, product formation needs
to be monitored additionally after induction.
3.3.1
Biomass
Determination
Biomass is quantified via optical density (OD600) and gravimetri-
cally by weighing the dry cell weight (DCW) while flow cytometry
analysis (FCM) was used for the determination of cell death.
OD600 Determination
1. Any photometric device/plate reader quantifying the absorp-
tion in liquid broth can be used, e.g., a Genesys 20 photometer
(Thermo Scientific, Waltham, MA, USA).
2. Vortex fermentation broth after sampling to get homogenous
solution for 5–10 s.
3. Determine OD600 using photometric cuvettes within the linear
range of the system (i.e., 0.2–0.8 [AU]).
4. In case the sample is not measured within linear range, dilute
sample after vortexing with deionized water; make sure to
never exceed 1:10 dilution steps due to accuracy.
5. Conduct at least duplicate measurements.
DCW Determination
1. Preheat 2-mL Safe-Lock Tubes (e.g., Eppendorf, Hamburg,