3.7
Termination of
Experiment
1. After 96 h of cultivation, stop the perfusion, take out the grafts
and divide them into five equal samples by equidistant cross-
sectional cutting in order to perform the immune stainings and
AcLDL assay.
2. Store the graft sections in PBS and immediately proceed with
the assay and staining procedures.
3. The samples which are not used for AcLDL uptake assay should
be washed in PBS (in 50 ml falcon tube) for 5 min, followed by
fixation with in 4% PFA for 5 min (in 15 ml Ficoll tube). Wash
them twice afterwards in an excess volume of PBS in a 50 ml
falcon tube.
3.8
AcLDL Uptake
Assay (Modified from
Manufacturer’s
Instructions)
The AcLDL assay is an easy and direct method to verify the intact
functionality of the seeded endothelial cells by the uptake of acety-
lated low density lipoprotein (LDL) particles via scavenger recep-
tors expressed on an functionality intact endothelial cell [21]. As a
result, positive signals would indicate an unimpaired function of the
endothelial cells, while the lack of LDL signals would indicate
either impaired and degenerated endothelial cells or might repre-
sent a possible overgrowth by non-endothelial cells.
1. Place
one
of
the
samples
from
3.7.2
in
a
2
ml
microreaction tube.
2. Wash the designated sample two times with PBS+.
3. Cover the sample in an excess of AcLDL working solution. The
working solution consists of the respective cell culture medium
with 10% FCS and 1.25% (v/v) AcLDL supplied stock solu-
tion. For 1 cm of sample, we used 400 μl of AcLDL working
solution.