Yannick Nossin1, Eric Farrell2, Wendy J L M Koevoet1, Frank Datema1, Rodrigo A Somoza3,4, Arnold I Caplan3,4, Gerjo J V M van Osch1,5,6. 1. Department of Otorhinolaryngology, Erasmus MC, University Medical Center Rotterdam, Rotterdam, the Netherlands. 2. Department of Oral and Maxillofacial Surgery, Erasmus MC, University Medical Center Rotterdam, Rotterdam, the Netherlands. 3. Department of Biology, Skeletal Research Center, Case Western Reserve University, Cleveland, OH, USA. 4. CWRU Center for Multimodal Evaluation of Engineered-Cartilage, Cleveland, OH, USA. 5. Department of Orthopaedics, Erasmus MC, University Medical Center Rotterdam, Rotterdam, the Netherlands. 6. Department of Biomedical Engineering, Faculty of Mechanical, Maritime, and Materials Engineering, Delft University of Technology, Delft, the Netherlands.
Abstract
OBJECTIVE: Cartilage is avascular and numerous studies have identified the presence of single anti- and pro-angiogenic factors in cartilage. To better understand the maintenance hyaline cartilage, we assessed the angiogenic potential of complete cartilage releasate with functional assays in vitro and in vivo. DESIGN: We evaluated the gene expression profile of angiogenesis-related factors in healthy adult human articular cartilage with a transcriptome-wide analysis generated by next-generation RNAseq. The effect on angiogenesis of the releasate of cartilage tissue was assessed with a chick chorioallantoic membrane (CAM) assay as well as human umbilical vein endothelial cell (HUVEC) migration and proliferation assays using conditioned media generated from tissue-engineered cartilage derived from human articular and nasal septum chondrocytes as well as explants from bovine articular cartilage and human nasal septum. Experiments were done with triplicate samples of cartilage from 3 different donors. RESULTS: RNAseq data of 3 healthy human articular cartilage donors revealed that the majority of known angiogenesis-related factors expressed in healthy adult articular cartilage are pro-angiogenic. The releasate from generated cartilage as well as from tissue explants, demonstrated at least a 3.1-fold increase in HUVEC proliferation and migration indicating a pro-angiogenic effect of cartilage. Finally, the CAM assay demonstrated that cartilage explants can indeed attract vessels; however, their ingrowth was not observed. CONCLUSION: Using multiple approaches, we show that cartilage releasate has an inherent pro-angiogenic capacity. It remains vessel free due to anti-invasive properties associated with the tissue itself.
OBJECTIVE: Cartilage is avascular and numerous studies have identified the presence of single anti- and pro-angiogenic factors in cartilage. To better understand the maintenance hyaline cartilage, we assessed the angiogenic potential of complete cartilage releasate with functional assays in vitro and in vivo. DESIGN: We evaluated the gene expression profile of angiogenesis-related factors in healthy adult human articular cartilage with a transcriptome-wide analysis generated by next-generation RNAseq. The effect on angiogenesis of the releasate of cartilage tissue was assessed with a chick chorioallantoic membrane (CAM) assay as well as human umbilical vein endothelial cell (HUVEC) migration and proliferation assays using conditioned media generated from tissue-engineered cartilage derived from human articular and nasal septum chondrocytes as well as explants from bovine articular cartilage and human nasal septum. Experiments were done with triplicate samples of cartilage from 3 different donors. RESULTS: RNAseq data of 3 healthy human articular cartilage donors revealed that the majority of known angiogenesis-related factors expressed in healthy adult articular cartilage are pro-angiogenic. The releasate from generated cartilage as well as from tissue explants, demonstrated at least a 3.1-fold increase in HUVEC proliferation and migration indicating a pro-angiogenic effect of cartilage. Finally, the CAM assay demonstrated that cartilage explants can indeed attract vessels; however, their ingrowth was not observed. CONCLUSION: Using multiple approaches, we show that cartilage releasate has an inherent pro-angiogenic capacity. It remains vessel free due to anti-invasive properties associated with the tissue itself.
Cartilage is an avascular tissue and the absence of blood vessels is considered
a key feature in the homeostasis of permanent cartilage.
Healthy adult cartilage is often assumed to be anti-angiogenic in
nature. Indeed, it was shown that cartilage explants or tissue-engineered
cartilage constructs from adult chondrocytes are not invaded by blood
vessels and retains its stable cartilage phenotype when implanted
subcutaneously in mice.[2,3] Eisenstein and
colleagues have demonstrated that cartilage inhibits vessel invasion
due to factors that can be extracted from the tissue with guanidine hydrochloride.
Since components in this extracted fraction could be a useful tool
against cancer (anti-invasion factors),[6,7] this further
prompted search for specific proteins in cartilage that conferred the tissue
with this anti-angiogenic capacity and led to the identification of
proteins, such as chondromodulin and endostatin, that prevented vessel
formation and invasion.[6-13]However, cartilage does become invaded with blood vessels and can undergo
endochondral ossification in early stages of limb development or when its
integrity is disrupted as seen in osteoarthritis (OA).[14,15]
Most works studying the progression OA have found prevalent pro-angiogenic
factors, most notably one of the best-known factors driving angiogenesis,
vascular endothelial growth factor (VEGFa).
Interestingly, VEGFa is not only expressed in OA cartilage but also
in mature healthy cartilage and chondrocyte-derived tissue-engineered
constructs[17-19] that will not be
invaded by blood vessels. A pro-angiogenic potential of cartilage has been
observed in experiments with chondrocytes forming networks in
vitro in Matrigel[20,21] and with
conditioned medium of cultured chondrocytes on human umbilical vein
endothelial cell (HUVEC) proliferation, migration, and tube formation
in vitro.These apparent discrepancies reported in the literature about pro- and
anti-angiogenic properties of articular cartilage led us to question the
true angiogenic potential of cartilage. We set out to analyze the
angiogenesis regulating gene expression of cartilage, and performed
functional assays in vitro and in vivo to
evaluate the angiogenic effect of factors released from tissue engineered
cartilage as well as cartilage explants.
Methods
Generation of Conditioned Medium from Cartilage Explant and
Tissue-Engineered Constructs
Articular cartilage was obtained from 6 patients (3 males, 3 females, age
63-86 years) undergoing total knee replacement surgery with implicit
consent of the use of leftover material after surgery (after approval
by local ethics committee; MEC-2004-322). Cartilage was taken from
macroscopically unaffected areas. Nasal cartilage was obtained from 7
patients (3 males, 4 females, age 17-65 years) undergoing septal
corrections with implicit consent. Perichondrium was removed from
nasal cartilage with a scalpel. Four nasal septal cartilage donors
were utilized for chondrocyte isolation (2 males, age 58-65 years; 2
females, age 17-21 years). To isolate chondrocytes, harvested
cartilage was treated with 2 mg/mL protease B in physiological saline
solution (Sigma-Aldrich, St. Louis, MO, USA) for 90 minutes and
subsequently digested overnight in basal medium (Dulbecco’s modified
Eagle medium [DMEM], 4.5 g/L glucose with 10% fetal calf serum [FCS],
50 µg/mL gentamicin, and 1.5 µg/mL fungizone [all Invitrogen,
Carlsbad, CA, USA]) supplemented with 0.12 U collagenase B (Roche
Diagnostics, Almere, the Netherlands). The resulting primary
chondrocytes were seeded at a density of 7,500 cell/cm2 in
T175 culture flasks for expansion with the above-mentioned basal
medium. For generation of stable cartilage pellets, articular
chondrocytes at passage 1 and nasal chondrocytes at passage 3 were
utilized.Pellet cultures of chondrocytes were formed by seeding 2.0 ×
105 cells in 0.5 mL in a 15-mL conical polypropylene
tube and centrifuging for 8 minutes at 300 × g.
Pellets from both cell sources were cultured in normoxic conditions
for 21 days in chondrogenic medium (high-glucose DMEM with 50 μg/mL
gentamicin [Invitrogen], 1.5 μg/mL fungizone ([nvitrogen], 1 mM sodium
pyruvate [Invitrogen], 40 μg/mL proline [Sigma, Kawasaki, Kanagawa
Prefecture, Japan], 1:100 v/v insulin-transferrin-selenium [ITS; BD
Biosciences, San Jose, CA, USA], 10 ng/mL transforming growth factor
β1 [TGFβ1; R&D Systems], 10 mM ascorbic acid-2-phosphate [Sigma],
and 100 nM dexamethasone [Sigma]). The medium was renewed twice a
week. At day 21, medium was renewed and 24 hours later the pellets
were washed with phosphate buffered saline (PBS) and incubated with
basal medium consisting of phenol-red free DMEM (Gibco, Waltham, MA,
USA) with 0.1% w/v bovine serum albumin (BSA; Sigma) and 10 mM
ascorbic acid-2-phosphate (Sigma) for 24 hours to produce conditioned
medium (CM) for downstream experiments. This CM was collected, cell
debris removed by centrifugation at 300 × g for 8
minutes and stored at −80 °C. Pellets were digested in 350 μL RNABee
(Tel-Test, Inc., Pearland, TX, USA) and stored at -80°C for subsequent
gene expression analysis. Additional pellets were fixed in 4% formalin
at room temperature overnight and then processed for histological
analysis.To generate CM from tissue explants we used nasal septal cartilage (3
donors) and 3 bovine fetlock joints as source for hyaline cartilage.
After determining their weight and washing with basal medium, the
explants were placed per 100 mg of tissue in 1 ml of basal medium.
After 24 hours the CM was collected, cell debris removed by
centrifugation at 300 × g for 8 minutes and stored at
−80 °C.
Identification of Angiogenesis Regulating Genes in RNAseq
Dataset
To identify known angiogenesis regulating factors expressed by human
adult articular cartilage using a dataset generated previously
(GSE128554). More details can be found in the Supplemental Material. The data were compared with
Gene Ontology and Uniprot data regarding: angiogenesis (GO:0001525)
604 genes, negative regulation of angiogenesis (GO:0016525) 91 genes,
as well as positive regulation of angiogenesis (GO:0045766) 218
genes.
Gene Expression Analysis
To isolate RNA, the pellets in RNABee were homogenized with an Eppendorf
Micro-pestle (Eppendorf, Hamburg, Germany). Total RNA isolation was
performed utilizing the RNeasy Column system (Quiagen, Hilden,
Germany). 0.5 μg RNA was used for cDNA synthesis using the RevertAid
First Strand cDNA kit (Thermo Fisher, Waltham, MA, USA). Gene
expression was analyzed by real-time reverse transcription
quantitative polymerase chain reaction (RT-qPCR) on a StepOnePlus
System using SYBR Green (Applied Biosystems, Foster City, CA, USA) or
Taqman (Thermo Fisher) assays. Primer and probe sequences in the
supplementary materials. The best housekeeper index
(BKI) was calculated from GAPDH,
RSP27, and HPRT.
Histology
Fixed pellets were paraffin embedded and sectioned. Deposition of
glycosaminoglycan (GAG) was determined by thionine staining.For immunohistochemical stainings, sections were pretreated with 0.1% w/v
pronase and 1% w/v hyaluronidase and blocked using normal goat serum
(Southern Biotech, Birmingham, AL, USA). Sections were incubated with
either mouse monoclonal antibody against collagen type II 0.4 μg/mL
(Developmental Studies Hybridoma Bank, Cat. #II-II6B3) for 60 minutes
or collagen type X 5 μg/mL (ThermoFisher, Clone X53, Cat. #14-9771-82)
in PBS 1% BSA overnight. After incubation with a biotinylated goat
anti-mouse antibody and ALP-conjugated streptavidin, staining was
revealed by incubation with a New Fuchsin substrate (Chroma, Kongen,
Germany). As corresponding isotype controls 0.4 μg/mL and 5 μg/mL of
an isotype immunoglobulin G1 monoclonal antibody were used.
Angiogenesis Assays
Commercially derived pooled HUVEC (Lonza, Basel, Switzerland) were seeded
at a density of 5 × 103 cells/cm2 in culture
flasks and cultured in endothelial growth medium (EGM-2 Promocell,
Heidelberg, Germany). The medium was renewed every 2 to 3 days. When
they neared confluency, cells were detached with 0.05 % trypsin-EDTA
(Gibco) and used for angiogenesis assays. For angiogenesis assays,
HUVECs between passages 8 and 10 were used.
Endothelial Cell Migration Assay
Migration assays were performed by seeding HUVEC (5 × 104
cells/well) in 24-well Transwell inserts (8 µm pore size, Corning Life
Sciences, Corning, NY, USA) in serum-free medium containing 0.05% BSA
(Merk, Kenilworth, NJ, USA). The different CMs were placed in the
lower compartment of different wells and diluted 1:1 with endothelial
basal medium (EBM-2, Promocell). EBM and unconditioned medium (UCM)
were used as negative controls and EGM-2 was used as positive control.
After 10 hours of incubation at 37 °C and 5% CO2, the cells
on the membrane were fixed with 4% formaldehyde/PBS and the
nonmigrated cells from the upper surface of the membrane were removed
with a cotton swab. We confirmed that no cell proliferation took place
during the 10-hour incubation, based on cell count. The migrated cells
were then stained with DAPI (4′,6-diamidino-2-phenylindole) and then
quantified by fluorescence microscopy and image analysis through
ImageJ utilizing the included particle analysis macro. Five
nonoverlapping pictures were taken and the average cell count per well
for three independent experiments was calculated.
Endothelial Proliferation
To measure proliferation, 2.5 × 103 HUVEC/cm² were seeded in
48-well plates. After 24 hours, the medium was replaced with EBM to
synchronize the cells. After 8 hours, the cells were stimulated with
CM, EGM-2 as positive control, or EBM-2 as negative control for 24
hours. With the stimulus, 10 µM dEdU (d-5-ethynyl-2′-deoxyuridine;
BaseClick, Neuried, Germany) was added to stain DNA of replicating
cells. After 24 hours, the cells were washed with PBS and fixed with
4% formalin for 5 minutes. The EdU-label was revealed utilizing the
manufacturers protocol. The cells were counterstained with DAPI and
imaged using fluorescence microscopy. Utilizing the particle analysis
macro in ImageJ, we determined the average amount of positively
stained cells per image for DAPI and EdU and the percentage of cells
positive for EdU was calculated.
Chick Chorioallantoic Membrane Assay
Fertilized chicken eggs laid the day before (purchased from Drost
Loosdrecht B.V., Netherlands) were incubated sideways at 37 °C and 65%
humidity for 3 days before rupturing the air-sack and opening a small
hole on the top to deflate the air-sack. At day 7 of incubation, part
of the shell was removed to start the assay. CM was concentrated
20-fold using Amicon Ultra-2 mL Centrifugal Filters (Merck,
Kenilworth, NJ, USA). One sterile filter disk (5 mm diameter) soaked
with 5 µL concentrated CM was placed on the chorioallantoic membrane
(CAM) of the egg. Concentrated basal medium was used as negative and
100 ng FGF2 was used as positive control.
After 3 days of incubation, the CAM was fixed with 4% formalin
and removed from the egg. Induction of vessel formation was assessed
by 3 independent observers ranking blinded 45 pictures for the amount
of attracted vessels and their directionality toward the stimulus.Eight bovine cartilage explants (5 mm diameter) were placed on filter
rings on the CAM of 8 separate eggs. After 7 days of incubation the
tissue and surrounding CAM were fixed with 4% formalin for 24 hours,
imaged, and subsequently processed for histology.
Data Analysis and Statistics
Before each statistical test the data were evaluated for normal
distribution via descriptive statistics as well as visual inspection
and subsequently the appropriate tests were chosen. The in
vitro angiogenesis assays were statistically evaluated
with a linear mixed model (experimental conditions as fixed factor,
repeats as random factor) with Bonferroni post hoc
correction. For articular chondrocytes constructs 2 batches of CM
created by pooling 3 donors were tested in triplicate in independent
experiments. For the cartilage explant derived CM as well as the nasal
chondrocyte constructs CM of each donor was tested separated in
triplicate. For the CAM assay, the interobserver correlation was
tested through a Spearman correlation test. The conditions were
compared using the average rank of 3 observers with a Mann-Whitney
U test. Data are described as mean and standard
deviation. The positive controls, included to be able to exclude
technical failures, were calculated separately from statistical
analyses. Statistical analysis was performed using SPSS 11 for Windows
(IBM, Armonk, NY, USA).
Results
Gene Expression Analysis Revealed Plethora of Pro-Angiogenic Genes
Expressed by Healthy Adult Cartilage
In healthy adult human articular cartilage 385 of the total 15032
expressed genes were associated to regulation of angiogenesis or
vasculogenesis. Of these 385 genes 63 genes were associated with the
negative regulation of angiogenesis and 116 were known pro-angiogenic
genes of which most are more highly expressed than d21 chondrogenic
differentiated mesenchymal stem cells (MSCs)
(
).Expression of angiogenesis regulating genes in human adult
articular cartilage. Table depicts the angiogenesis
regulating fraction of the top 1000 highest expressed
human adult articular cartilage (HAAC) genes as well the
average of chondrogenically differentiated mesenchymal
stem cells (MSCs) of 3 donors as a known pro-angiogenic
condition for comparison. FPKM = fragments per kilobase of
transcript per million mapped reads.
Releasate of Tissue-Engineered Cartilage Constructs Promoted
Endothelial Cell Proliferation and Migration In Vitro
and Angiogenesis In Vivo
The tissue-engineered cartilage from human articular chondrocytes stained
positive for glycosaminoglycans and type II collagen, confirming
cartilage tissue formation (
). Chondrogenic phenotype was further confirmed by high gene
expression of chondrogenic marker COL2A1 and a very
low or absent expression of the hypertrophic markers
COL10A1 and ALPL. (
). To assess the effects of CM on specific aspects of
angiogenesis, we performed an endothelial cell proliferation assay
using EdU incorporation. The CM induced a 3.1-fold (±2.1) increase
(P = 0.028) in the number of cells
proliferating compared with the non-CM (
and
). To evaluate the effect of CM on endothelial cell migration
we used a modified Boyden chamber assay. Exposure to CM resulted in
4.5-fold (±2.4) (P = 0.0004) increased number of
migrated cells, indicating factors released by chondrogenically
redifferentiated human articular cartilage derived constructs increase
endothelial cell migration (
and
). The CM derived from the cartilage constructs attracted
significantly (P = 0.006) more vessels than UCM in
the CAM assay (
and
). The collected CM from tissue-engineered construct of human
nasal septal chondrocytes (
) demonstrated a pro-angiogenic effect, similarly to the
constructs from articular chondrocytes. In the in
vitro assays the nasal chondrocyte construct releasate
induced a 7.0-fold (±3.2) (P = 0.000017) increase in
endothelial proliferation (
) and 4.5-fold (±2.7) (P = 0.005) increase in
endothelial migration (
). Looking at the complete process of vessel formation in the
CAM assay we observed significantly more vessels clearly directed
toward the filter disks with CM of nasal septal chondrocytes than with
the UCM (
). To confirm that the CAM assay was suitable to show
anti-angiogenic effects we added a control with a blocking antibody of
VEGFa. In summary, these results demonstrate that the releasate of
chondrocytes derived from hyaline cartilage (articular and septal) is
pro-angiogenic.Pro-angiogenic effect of conditioned medium from
cartilaginous tissue generated from culture expanded human
articular chondrocyte. (A) Histological and
immunohistological staining of day 21 chondrogenically
redifferentiated chondrocyte pellets of 3 donors for
thionine (first row) and collagen type II (second row).
(B) Quantitative polymerase chain
reaction (qPCR) gene expression analysis of chondrogenic
and hypertrophy marker genes showing the mean and SD of 3
donors. Cutoff value for expression Ct = 35, BHK = best
housekeeper index calculated from GAPDH, RSP27, and HPRT1.
(C) Endothelial proliferation assay,
showing in cyan positive EdU staining, counterstained with
DAPI (blue). (D) Quantification of
proliferating HUVECs after 24 hours. (E)
Endothelial migration assay. (F)
Quantification of number of migrated cells.
(G). Chick chorioallantoic membrane
with CM-soaked filter disks. (H) Ranking of
CAM assay (lowest =1 highest =15: average of 3 independent
observers; box = interquartile range, whiskers +1%-99%)
N = 6 per condition, performed with
2 batches of CM (each batch is represented by different
symbols). EdU, 5-ethynyl-2′-deoxyuridine; DAPI,
4′,6-diamidino-2-phenylindole; CM, conditioned medium;
CAM, chick chorioallantoic membrane; HUVEC, human
umbilical vein endothelial cell.Chondrogenic redifferentiation of nasal septal chondrocytes
releasate acts pro-angiogenic. (A)
Histological and immunohistological staining of day 21
chondrogenically differentiated nasal chondrocytes for
collagen type II, thionine, and collagen type X.
(B) Quantitative polymerase chain
reaction (qPCR) gene expression analysis of chondrocyte
and hypertrophy marker genes showing the average and SD of
3 donors. Cutoff value for expression Ct = 35.
(C) Quantification of number of
proliferating cells. 2 experiments with a total of 4
separate donors done in triplicate. (D)
Quantification of number of migrated cells. Two
experiments with a total of 4 separate donors done in
triplicate. (E) Vessel rank of chick
chorioallantoic membrane (CAM) assay: higher rank = more
pro-angiogenic. Four donors with n =
5.
Releasate of cartilage explants stimulated pro-angiogenic
effect
The CM of bovine articular cartilage and human nasal septal cartilage
were evaluated in vitro for their effect on migration
and proliferation of HUVEC and in vivo on a CAM assay (
). The bovine articular cartilage–derived CM, increased
proliferation 4.24-fold (±0.60) (P = 0.0000002) (
) and migration 6.1-fold (±2.36) (P = 0.0001)
of endothelial cells (
). The nasal cartilage–derived medium led to a 3.43-fold
(±0.95) (P = 0.00001) increase in endothelial
proliferation (
) and a 6.06-fold (±2.36) (P = 0.002) increase
in endothelial migration (
). Finally, the CAM assay confirmed this pro-angiogenic
capacity of the releasate of cartilage explants as reflected by an
increased attraction of vessels (
and
), albeit only with the bovine articular cartilage derived CM
the effect was statistically significant.The releasates of healthy bovine articular cartilage and
human nasal septal cartilage are pro-angiogenic.
(A) Histology of bovine articular
cartilage stained with thionine. (B)
Histology of human nasal septal cartilage stained with
thionine. (C) Endothelial cell proliferation
with articular cartilage tissue–derived CM.
(D) Endothelial cell migration with
articular cartilage tissue derived CM. (E)
Endothelial proliferation with nasal cartilage
tissue–derived CM. (F) Endothelial cell
migration with nasal cartilage tissue–derived CM.
(G) CAM vessel rank with articular
cartilage–derived CM. (H) CAM vessel rank
with nasal cartilage tissue–derived CM. Higher rank = more
pro-angiogenic. Statistical evaluation of the in
vitro assays was done utilizing a linear
mixed model with Bonferroni post hoc test
(chondrocyte donors are represented with separate symbols,
while the separate experiments are represented via the
filling of the symbols). CM, conditioned medium; CAM,
chick chorioallantoic membrane.After the CM approach, we repeated the original set-up used by Eisenstein
and colleagues
using cartilage explants and cartilage tissue extracts. After a
week of incubation of viable bovine articular cartilage explant on the
CAM, we confirmed their observations that vessels did not penetrate in
the cartilage (
); however, we saw a trend toward blood vessel attraction (
). Additionally, we extracted bovine articular cartilage with 4
M guanidine HCl. As in the experiments of Sorgente et
al.,
the dialyzed extract of bovine articular cartilage indeed
inhibited blood vessel attraction in the CAM assay (
).Bovine articular cartilage tissue shows a pro-angiogenic
trend in the chick chorioallantoic membrane (CAM) assay.
(A) Cartilage explants on the CAM,
showing vessel attraction. (B) Representative
sections of 1 of 8 cartilage explants after 7 days of
incubation. (C) Dialyzed cartilage extracts
on the CAM, showing inhibition of vessel formation.
Pictures depict different donors of the shown
conditions.
Discussion
In this study, we demonstrated that the cartilage releasate is overall
pro-angiogenic. This pro-angiogenic effect was proven with releasate from
tissue-engineered cartilage from cultured human articular and nasal
chondrocytes as well as cartilage explants of human nasal cartilage and
bovine articular cartilage using in vitro assays for
endothelial cell proliferation and migration as well as the CAM in
vivo assay. Finally, we repeated the initial experiment
described by Eisenstein et al. in which cartilage explants
were used in the CAM assay and we confirmed their findings that cartilage
tissue itself is not invaded by vessels. In fact, we could demonstrate that
it did attract vessels. In addition, we confirmed that high salt extracts of
cartilage were indeed anti-angiogenic. In combination with our gene
expression data of adult cartilage we demonstrated a pro-angiogenic property
of the cartilage releasate and showed that cartilage behaves like every
other hypoxic tissue, however it has an additional anti-invasive property
found in the tissue itself, possibly associated to cartilage matrix
intrinsic properties or matrix bound factors.We first determined the source of the common understanding that cartilage is
anti-angiogenic. Early publications already described cartilage as a
vessel-free tissue.
The landmark series of publications contributing to the perception of
cartilage as a tissue preventing vessel invasion was the 3-part series of
“Tissues Resistant to Vascular Infiltration, I-III” published by the group
of R. Eisenstein,[4,5,27] in which cartilage was shown to prevent vessel
invasion and cartilage extract was shown to prevent endothelial
proliferation. This was further cemented by Folkman et al.[8,9]
demonstrating that cartilage, and its dialyzed high salt extract, has
relevance for the development of anticancer drugs. In search for factors
preventing angiogenesis to use in cancer therapy the line between
anti-invasive factors and anti-angiogenic factor became blurred and led to
cartilage being commonly accepted as being anti-angiogenic.[1,6-8,10-12,29-32]
We confirmed that cartilage explants are not invaded by blood vessels in the
CAM assay and that a high salt extract of cartilage matrix inhibited blood
vessel attraction. However, our results demonstrated that although not
invaded, cartilage explants do attract vessels, indicating that its
releasate is pro-angiogenic. The anti-angiogenic effects of high salt
extract of cartilage are most likely due to released matrix-bound factors,
which seem to be anti-angiogenic, as shown in the extract experiment (
), showing the anti-invasive characteristics of cartilage. Differing
from the many publications that identified anti-angiogenic factors in
cartilage,[12,33-36] are the studies
on osteoarthritis that showed pro-angiogenic properties of
cartilage.[15,17,37-41] Following these
results, we found that pro-angiogenic properties of cartilage have been
reported as early as the first publication of Eisenstein et
al.
Further studies supported this hypothesis, demonstrating the presence
of VEGFa in mature articular cartilage, via gene expression or ELISA
(enzyme-linked immunosorbent assay) analyses in the secretome.[17,18]
This is also reflected in the pro-angiogenic behavior observed in in
vitro assays,[20,42] although this
behavior was ignored because the main goal of that study was to show an
increased angiogenesis during OA. In our RNAseq dataset, we observed that,
next to known anti-angiogenic genes, many pro-angiogenic genes were highly expressed.
This comes with the caveat that there are currently more known
pro-angiogenic than anti-angiogenic genes, which might skew the selection
toward pro-angiogenic genes. The identified pro-angiogenic genes, however,
are highly expressed and well-established mediators of vessel formation and
attraction such as VEGFa, HIF1a, and
FGF1, strengthening the conclusion of a potential
pro-angiogenic effect of the cartilage releasate. Our selection of the top
1000 genes was made arbitrarily with the intention to focus on high
expressed genes and only to get an insight into the distribution of
angiogenesis regulating genes, explaining the absence of well-known
anti-angiogenic genes which were lower expressed. Furthermore, the
expression of many other genes leads us to hypothesise that the observed
pro-angiogenic effect is explained by a combination of factors.The most commonly used angiogenesis assays are based on the effects observed in
HUVECs, which are commonly used as a model system to study subprocesses of
vessel formation.
Endothelial cell migration and proliferation mimic the first steps of
the formation of a new vessel starting from an existing one, while the
network forming assay or tube-forming assay displays the potential of
completely new vessel formation. Altogether, these assays can provide a
broad picture of the angiogenic effect of a specific factor or the whole
releasate; however, they only reflect the effects of single cellular
functions and do not reflect the cellular interplay needed in the complex
process of vessel formation. To evaluate the effect of cartilage-released
factors on a fully functional, mature vessel we utilized the CAM assay. This
technique allows to observe the effect of different factors on the entire
process of angiogenesis, from the disruption of a mature vessel to the
formation, direction, and maturation of a new vessel. Overlapping multiple
angiogenesis assays that span the entire vessel development process, we were
able to confirm that the effects we observed in vitro are
also observed in vivo. These results strengthened our
conclusion that the cartilage releasate is pro-angiogenic.We demonstrate that the releasate from both human articular and nasal
chondrocytes-derived cartilage, was pro-angiogenic. Importantly, we
previously shown that the cartilage derived from both types of chondrocytes
remains stable (i.e., it does not get ossified) after in
vivo implantation.[2,3] The articular
cartilage used for this study was obtained from total knee replacement
surgeries, and although exclusively macroscopically, not diseased-affected
sections were harvested, there are indications that this cartilage may
contains cells with a hypertrophic phenotype.
To address this issue, we also utilized nasal septal cartilage
derived chondrocytes, a hyaline cartilage source, free of osteoarthritis,
which confirmed the pro-angiogenic capacity of hyaline cartilage. To exclude
a possible effect of TGFβ in the pro-angiogenic behaviour of the tissue
engineered constructs,
we also tested CM derived from the native cartilage tissue and
demonstrated that both releasates induce a pro-angiogenic response. This
effect was independent of the source of the tissue, as we tested both human
nasal cartilage as well as bovine articular cartilage and when compared to
previously published data it has a similarly pro-angiogenic effect as d21
chondrogenically differentiated.
Experiments with cartilage explants on CAM further confirmed the
secretion of factors that attracted blood vessels, clearly showing that the
releasate of cartilage is not anti-angiogenic.Besides showing that the releasate from cartilage and chondrocyte- derived
constructs is pro-angiogenic, we also demonstrated that the apparent
anti-angiogenic nature of cartilage is probably related to the matrix. With
the common conception that articular cartilage turns pro-angiogenic during
OA, a common approach has been to utilize anti-angiogenic treatment options.
Our results suggest that the permissive invasion of blood vessels in
OA might not be due to the presence of soluble factor(s), but instead might
associated with specific cartilage matrix or matrix-bound factors. This
could direct more attention to study the effects of cartilage integrity on
blood-vessel invasion. For cartilage regeneration strategies it will be key
to consider the replacement of this barrier function and to study the
effects of the extracellular matrix for the possible role of extractable
anti-angiogenic factors in cartilage repair and regeneration. Reproducing
both on top of a mature chondrocyte phenotype, seem to be key to manufacture
stable cartilage. This work is meant to supplement the already broad list of
angiogenesis-related cartilage literature and to clarify the
misunderstandings about the anti-angiogenic nature of cartilage that exist
in the field. This information might be of value for further research on the
embryonic development of cartilage and bone, the progression of OA and
tissue engineering.Click here for additional data file.Supplemental material, sj-pdf-1-car-10.1177_19476035211047628 for The
Releasate of Avascular Cartilage Demonstrates Inherent Pro-Angiogenic
Properties In Vitro and In Vivo by Yannick Nossin, Eric Farrell, Wendy
J.L.M. Koevoet, Frank Datema, Rodrigo A. Somoza, Arnold I. Caplan and
Gerjo J.V.M. van Osch in CARTILAGE