3. Following the coating procedure, remove the remaining
Synthemax™II-SC working solution from the T75-Flask and
add the 20 mL of pre-warmed cell culture medium.
4. Expand the hASC cells (see Note 5) in T75-Flasks to produce
enough cells to inoculate the desired cultivation systems.
(a)
Thaw the hASC cells at least 7 days prior to their expan-
sion in the stirred systems. Remove one cryovial contain-
ing approximately 1 mL cell suspension with a density of
at least 1 � 106 cells mL�1 from the cryogenic storage
tank and immediately thaw the vial in a pre-warmed water
bath (37 �C). Prevent the lid from touching the surface of
the water bath to prevent contamination. As soon as only
small ice crystals are left, wipe the vial down with a tissue
soaked in ethanol. The entire contents of the cryovial
should be transferred to the T75-Flask, containing the
pre-warmed media, under sterile conditions to achieve a
final cell density of 50,000 cells mL�1 (or approximately
13,333 cells cm�2).
(b)
Incubate the cells under static conditions at 37 �C, 5%
CO2, and 80% relative humidity for 6 h (see Note 7).
(c)
Following a 6 h incubation period, inspect the T75-Flask
under the microscope (see Note 1) and determine cell
attachment to the substrate. Once confirmed, replace the
supernatant with fresh pre-warmed cell culture media.
(d)
Monitor the T75-Flask by microscope every 24 h until the
cells achieve 80–90% confluency (see Note 1). At this
point, passage the cells (see Notes 9, 11, and 12) into
2–5 freshly coated T75-Flasks (see Note 8), depending on
the desired inoculum quantity. Inoculate each flask con-
taining 20 mL of pre-warmed culture medium (see Note
6), at a density of 10,000 cells cm�2.
(e)
Again, monitor the T75-Flasks every 24 h by microscope
until the cells have achieved 80–90% confluency (see Note
1). Subsequently, passage the cells (see Notes 9 and 11),
determine their cell density and quality (see Note 12),
then transfer the required cell quantity to the cultivation
systems of choice.
3.2
hASC Expansion
in Corning’s Spinner
Flasks
1. The following procedure describes the xeno- and serum-free
expansion of hASCs in chemically defined medium and 125 mL
spinner flasks (100 mL working volume) using a partial media
exchange approach. Approximately 24 h prior to the inocula-
tion of the spinner flasks, begin with preparations of the culture
medium, MCs, and spinner system.
(a)
Pre-warm at least 150 mL of cell culture medium (see
Note 6) to 37 �C for the expansion procedure per spinner
flask.
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Misha Teale et al.