(b)
Subsequently, transfer at least 1 g (¼ 360 cm2) of Pro-
Nectin® F MCs (see Note 10) per spinner flask to a
100 mL Schott Flask (Duran) and suspend them in sterile
Dulbecco’s phosphate-buffered saline (DPBS) to achieve
a final MC concentration of 100 g L�1. Autoclave the MC
suspension at 121 �C for 20 min.
(c)
Allow the suspension to cool to room temperature and the
MCs to sediment at the bottom of the flask. Remove and
discard the supernatant, while ensuring that no MCs are
lost in the process. Replace the discarded supernatant with
pre-warmed culture medium (see Note 13). Repeat this
step twice to obtain a sterile ProNectin® F MC stock
solution.
(d)
Transfer the packaging containing the spinner flask to the
biosafety cabinet. Open the package and assemble the
spinner flask under the bench using the appropriate tech-
nique to guarantee cultivation vessel sterility.
(e)
Add 90 mL of pre-warmed culture media (see Note 6) and
10 mL of ProNectin® F MC stock solution to the spinner
flask.
(f)
Transfer the spinner flask back to the incubator containing
the stirrer platform and allow the MCs to equilibrate
under process conditions, i.e., 37 �C, 5% CO2, 80% rela-
tive humidity and Ns1u (see Notes 7 and 14), for approxi-
mately 24 h prior to inoculation. This step also serves to
ensure vessel sterility prior to cultivation.
2. Inoculation of the spinner flask.
(a)
Calculate the necessary volume of inoculum, following
cell density and quality control (see Note 12), to achieve
an initial cell density of 15,000 cells cm�2 or 5.4 � 106
cells per spinner flask.
(b)
Transfer the equilibrated spinner flask to the biosafety
cabinet and allow the MCs to sediment. Subsequently
remove the top lid and place it stirrer side up within the
biosafety cabinet.
(c)
Remove the volume of culture medium to be replaced
with the inoculum and transfer it to a sterile 15-mL cen-
trifuge tube (Corning®). This sample may then be used to
determine the initial substrate and metabolite concentra-
tion within the spinner flask (see Note 3). Add the inocu-
lum to the spinner flask to achieve the target starting cell
density.
(d)
Transfer the spinner flask back to the incubator containing
the stirrer platform and set the agitation rate to Ns1u for
5 min (see Note 14). Subsequently, reduce the speed to
0 rpm and allow the cells to sediment and attach to the
MCs for 12 h.
Mesenchymal Stem Cell Expansion at Benchtop-Scale
95