Development of bioprocesses for animal cells has to deal with different bioreactor types and scales. Bioreactors might be intended for generation of cell inoculum and production, research, process development, validation or transfer purposes. During these activities, not only the difficulty of up- and downscaling might lead to failure of consistency in cell growth, but also the use of different bioreactor geometries and operation conditions. In such cases, the criteria for bioreactor design and process transfer should be carefully evaluated in order to avoid an erroneous transfer of cultivation parameters.In this work, power input, mixing time, impeller tip speed, and Reynolds number have been compared systematically for the cultivation of the human cell line AGE1.HN® within three partner laboratories using five different bioreactor systems. A common process window for mixing time in the range of 8 – 13 s has been found in bioreactors having significant differences in their inner geometries. The obtained results are employed for process standardisation and transfer between research institutions.
Cell culture in laboratory bioreactors with different inner geometries
Finding conditions for consistent cultivation of mammalian cells in bioreactors is not an easy task. For standard stirred tanks, correlations existing in literature can be used in order to predict operation conditions for process transfer purposes. However, if the inner geometry of two bioreactors cannot be compared within tolerance ranges, the characterization of the bioreactor hydrodynamics becomes necessary.For this work, five geometrically different bioreactors were used, which are operated within three partner laboratories for data generation during research on Systems Biology. Characterization of the bioreactor hydrodynamics was performed with the main goal of finding a relationship between process transfer criteria and cell growth in the systems.
Bioreactor characterization
Following criteria were considered for characterization of bioreactor hydrodynamics.(1) Power input ( Power numbers Np were calculated from Np = f(Re) correlations available in literature [1-3]. Corrections for Np were considered due to geometry deviations from a standard configuration [4-7]. Volumetric power inputs were calculated according to Equation 1:(2) Mixing time ( This criterion was obtained from the decolourization of a I/KI solution of after addition of Na. Starch was added previously to the bioreactor. Decolourization time course was video recorded. The resulting videos were computer analyzed, and Θ was obtained after gray-scale conversion and measurement of loss of saturation (MATLAB, MathWorks).(3) Impeller tip speed ( calculated according to Equation 2.(4) Reynolds Number at impeller tip ( calculated according to equation 3:The specific growth rate was employed as indicator for comparison of bioreactor performance. The use of μ made the comparison of the two cell line clones possible, despite the differences in initial cell densities during bioreactor culture.
Relationship between cell growth and process transfer criteria
Figure 1 shows the dependency of the μ on process transfer criteria. A process window for mixing time values between 8 and 13 seconds can be identified as common for all bioreactors, where the smallest deviation in µ between different bioreactors can be observed.
Figure 1
Relationship between maximum specific growth rate : a) Power input, b) Mixing time, c) Impeller tip speed, and d) Reynolds number. Curve fitting for bioreactors 3 (Black square) and 5 (Purple circle).
Relationship between maximum specific growth rate : a) Power input, b) Mixing time, c) Impeller tip speed, and d) Reynolds number. Curve fitting for bioreactors 3 (Black square) and 5 (Purple circle).
Conclusions
Criteria for process transfer were analyzed during the cultivation the human production cell line AGE1.HN. Growth was compared within ranges for power input, mixing time, impeller tip speed and Reynolds number. Maximum specific growth rates were observed for AGE1.HN cells at a common mixing time range of 8 - 13 seconds for all cultivation systems. This criterion was observed to be a reference for consistency of results within laboratory bioreactors with different internal geometry.Funding by the BMBF, Grand Nr. 0315275A is gratefully acknowledged.
Nomenclature
d impeller diameter [m]M degree of mixingN agitation speed [rpm]P = NpρN power input [W m-3]Re Reynolds number at impeller tip [-]u impeller tip speed [m s-1]V working volume [m3]
Greek letters
Θ mixing time [s]μ specific growth rate [d-1]ρ density [kg m-3]η dynamic viscosity [kg m-1 s-1]
Figure 1