system after rotational cell seeding, followed by low flow media-
perfusion for 5 days. The setup allows medium sampling and
describes the implementation of intraluminal cell proliferation and
functional assays to determine endothelial cell function and the
histological characterization of the seeded cell constructs. Next to
the 3D printed bioreactors, the system consists of common labora-
tory equipment such as pumps, filters and Luer Lock connectors
and is therefore easy to set up by common lab equipment.
It should be noted that today 3D printing has become an
affordable methodology that can be applied in many laboratories.
The above-mentioned methods can easily be adopted to tubular
vascular grafts with other dimensions by printing customized
bioreactors.
Thus, we describe an efficient, reliable, and affordable method
for evaluating the initial adherence and proliferation of endothelial
cells on tubular, acellular vascular grafts under in vitro dynamic
conditions.
2
Materials
2.1
Bioreactor Setup
The applied bioreactor was designed as a straight perfusion cham-
ber with two barb connectors for direct connection of the tubing
(from the outside) to the perfused grafts (on the inside) and recir-
culation of leaking medium.
1. Bioreactor chamber (see Note 1).
2. Tubing:
(a)
1 pump hose (PharMed BPT).
(b)
Silicon tubing (inner diameter 3 mm).
(c)
Female Luer Lock Style to barb connector (according to
used tubing diameters).
(d)
Male Luer Lock Style to barb connector (according to
used tubing diameters).
(e)
Y-connector 3–5 mm.
(f)
Three-way stopcock.
(g)
Sealing caps.
3. Syringes:
(a)
10 ml syringe with Luer Lock fitting.
(b)
50 ml syringe with Luer Lock fitting.
4. Reservoir bottle with three inlets and outlets for media trans-
port (see Note 2). We used a total of 50 ml of media for
approximately 2.5 cm2 of reseeded luminal surface area and
chose a 100 ml Schott Duran flask for reservoir.
In Vitro Colonization of Vascular Grafts
207