between various bioreactor scales. For the BioBLU® 0.3c, these
ratios are 0.5, 1.2, and 1.8 for d/D, HL/D, and H/D, respectively.
More information regarding the dimensions of the various com-
mercially available BioBLU® bioreactor types may be found on the
manufacturer’s website. Furthermore, due to the low stirrer instal-
lation height, high relative velocities are obtained near the bottom
of the reactor, which allows the suspension of MCs at low power
inputs and thus at acceptable hydrodynamic loads for the cells.
As previously mentioned, allogenic therapies require large
quantities of cells to treat multiple patients using a single universal
donor. This necessitates the use of pilot or production scale stirred
single-use bioreactors to achieve therapeutically relevant cell den-
sities in an economic and ecological manner. Due to the limitations
faced by spheroid-based cultures and the associated lack of process
reproducibility, this technique is of diminished importance here. In
contrast, the improved reproducibility when cultivating with MCs,
means their application, especially with regard to the production of
hMSCs for subsequent use in allogeneic therapies, is very popular.
Nevertheless, the same aspects (e.g., cell attachment, medium
composition), as described for the benchtop systems, apply at this
scale also. In their studies, Schirmaier et al. [37], Jossen et al.
[6, 38], and Lawson et al. [39] achieved maximum cell densities
of up to 0.7 � 106 cells mL�1 when cultivating in stirred pilot-scale
bioreactors (Biostat STR® 50 L and Mobius® CellReady 50 L) and
using cell culture medium supplemented with 10% human platelet
lysate and 5% fetal bovine serum (FBS), respectively. While it has
been shown that maximum cell densities (0.04–0.4 � 106 cells
mL�1) and expansion factors achieved in stirred bioreactors using
xeno- and serum-free cell culture media are still lower than those
achieved in serum-containing medium, a wide variety of new
serum-free media have recently come to market, paving the way
for higher hMSC densities to be achieved on production scale in
future.
1.2
Chemically
Defined, Serum-Free
Expansion of hMSCs
The most conventional cell culture media used for the production
of hMSCs are based on defined basal media, such as Dulbecco’s
Modified Eagle Medium (DMEM), Roswell Park Memorial Insti-
tute (RPMI) 1640, or Minimum Essential Medium (αMEM).
These basal media are subsequently supplemented with expensive
additives such as (a) proteins for cell adhesion, (b) lipids for cellular
anabolism, (c) growth factors and hormones to promote cell
growth, and in most cases, (d) an additional 10–20% (vol/vol)
FBS. While the disadvantages of serum addition (e.g., high batch-
to-batch variability, possible contamination with prions, viruses, or
zoonotic agents [40–44]) have been known for years, serum-
containing media are still used in many published academic studies
to this day. Meanwhile chemically defined, serum-free media not
only offer the advantage that all their components are known but
also that their quantities are stoichiometrically defined, facilitating
Mesenchymal Stem Cell Expansion at Benchtop-Scale
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