Masoumeh Eliyasi Dashtaki1, Masoud Hemadi1, Ghasem Saki2, Javad Mohammadiasl3, Ali Khodadadi4. 1. Cellular and Molecular Research Center, School of Medicine, Ahvaz Jundishapur University of Medical Sciences, Ahvaz, Iran. 2. Physiology Research Center, School of Medicine, Ahvaz Jundishapur University of Medical Sciences, Ahvaz, Iran. Electronic Address: ghasemsaki@yahoo.com. 3. Department of Medical Genetics, School of Medicine, Ahvaz University of Medical Sciences, Ahvaz, Iran. 4. Cancer, Environmental and Petroleum Pollutants Research Center, Ahvaz Jundishapur University of Medical Sciences, Ahvaz, Iran.
Infertility is among the common health issues
worldwide that affects 15% of couples. Among
infertile men, approximately 1% of the cases suffers
from obstructive or non-obstructive azoospermia,
with the latter being difficult to treat (1). One of the
causes involved in the non-obstructive azoospermia
is testicular torsion (2). Recently, researchers have
offered a new approach to the treatment of infertility
that involves differentiating stem cells into male
or female germ cells (3-6). Adipose tissue-
derived mesenchymal stem cells (AT-MSCs) have high
proliferation rate and self-renewal capacity, as well as
the potential to differentiate into various lineages (7).
Recent studies have shown that both embryonic and
adult stem cells are able to differentiate into primordial
germ cells (PGCs) and adult gametes (4, 8, 9). In 2006,
Nayernia et al. (4, 9) demonstrated the production of
a generation of mice from germ cells derived from
embryonic stem cells (ESCs) for the first time, and in
the same year, they were able to differentiate murine
bone marrow-derived MSCs (BM-MSCs) into germ
cells. Zhang et al. (10) recently reported that BM-
MSCs have the potential to trans-differentiate into
sperm-like cells, and can revive fertility in busulfantreated
azoospermic rats. Similarly, Cakici et al. (11)
have shown that AT-MSCs cause regeneration of
fertility in azoospermic rats.However, amongst the important issues for
therapeutic applications of these produced cells are
their low numbers and viability (12). To overcome these
problems, growth factors and several supplements are
often added to the culture media of these cells (13-15).
Epidermal growth factor (EGF) is a 53 amino acid
protein (16) involved in proliferation of spermatogonia
and regulation of spermatogenesis in mammalian testis
(17). It is also involved in the proliferation of MSCs
(14). Leukemia inhibitory factor (LIF) is involved in
the self-renewal process of stem cells, maintenance
of the non-differentiated forms of ESCs, MSCs, and
proliferation of PGCs (18, 19). The glial cell line-
derived neurotrophic factor (GDNF) is expressed by
glial cells in the brain (20), testicular and ovarian
tissues during the development, and it has been found
to be responsible for spermatogonial stem cells (SSCs)
self-renewal both in vitro and in vivo (21). The present
study is aimed to compare the performances of AT-
MSCs cultured with or without the addition of three
different growth factors EGF, LIF, and GDNF to their
culture medium, following their transplantation in
testicular torsion-detorsion mice.
Materials and Methods
Animals
In this experimental study, 6-8 week-old male Naval
Medical Research Institute (NMRI) mice were housed
under standard conditions (18-20°C and 12:12 hours light:
dark cycles) at the Research Center and Experimental
Animal House of Jundishapur University of Medical
Sciences (Ahvaz, Iran). All the experiments presented
in this study were approved by The Local Animal Care
Committees of Ahvaz Jundishapur University of Medical
Sciences (AJUMS) (IR.AJUMS.REC.2015.739), which
were in complete accordance with the guidelines for the
care and use of laboratory animals set by the national
academy of sciences (National Institutes of Health
Publication No. 86-23).
Isolation and culture of adipose tissue derived
mesenchymal stem cells
Adipose tissue was taken from epididymis of 5-10
male NMRI mice in a sterile environment. Then, the
samples were washed three times with phosphatebuffered saline (PBS, Gibco Life Technologies,
Paisley, UK) containing 3% penicillin/streptomycin(Pen/Strept) and 0.3% amphotericin B, then cut
into1-2 mm3 pieces. Blood vessels were removed fromthe tissue as much as possible and the pieces of fat
were incubated in collagenase type I enzyme (Sigma-
Aldrich, St. Louis, MO, 1 mg/ml) for 25-30 minutes at
37°C. To stop the enzyme activity, Dulbecco’s Modified
Eagle’s Medium (DMEM, Life Technologies, USA)
containing 10% fetal bovine serum (FBS, Gibco, Life
Technologies, USA) was added to the sample. The
suspension sample was centrifuged at 1200 rpm for 7
minutes, at room temperature and the cell pellet was
cultured in 25 cm2 flasks containing DMEM medium
supplemented with 15% FBS and 1% Pen/Strep, and
incubated at 37ºC in the presence of 5 % CO2. After
three days, the cell medium was replaced with fresh
medium and non-cohesive cells were removed. Medium
was changed once every two days until the cell density
reached 80-90%. The cells were then passaged for
more proliferation and purification. For this purpose,
1 ml 0.25% trypsin-ethylenediaminetetraacetic acid
(EDTA) was added to each flask and incubated for
2-3 minutes. When the cells were floating in the
flask, the trypsin was neutralized using 3-4 ml of the
medium containing FBS. Then, the cell suspension
was centrifuged for 7 minutes. at 1200 rpm and the
cell pellet was cultured in new flasks at a density of
20000/cm2 (22) .
MSCs are fibroblast analogue cells with adhesion
property and differentiation capacity (23). However,
before any transplantation it is necessary to confirm
the exact type of the cells isolated from donor animals.
For this purpose, we used the commonly applied flow
cytometry technique to confirm specific cell surface
markers on the cultured cells. The expression of CD90
and CD44 markers (specific to MSCs) and the lack of
expression of the two CD31 and CD45 markers (specific
to hematopoietic stem cells and endothelial cells) were
investigated, in our previous study (22).
In vitro osteogenic and adipogenic differentiation
potentials of adipose tissue-derived mesenchymal
stem cells
In order to further characterize of our cultured
cells, we assessed their ability to differentiate
into osteoblasts and adipocytes. For osteogenic
differentiation, AT-MSCs (passage 3) were cultured in
a 6-well plate (5×104 cells/well). After 24 hours, the
proliferative medium was replaced with osteogenic
differentiation medium [DMEM (low glucose), 10-7 M
dexamethasone, 50 µg/ml ascorbic acid , and 10 mM
B-glycerol phosphate (Sigma-Aldrich, St. Louis, Mo,
USA)]. The cells were incubated at 37°C and in 5%
CO2 for 21 days. Osteogenic medium was exchanged
every 3 days. At the end of the differentiation period,
AT-MSCs were fixed with 3% paraformaldehyde and
the presence of calcium deposits was examined using
0.5 % alizarin red solution.For adipogenic differentiation, 5×104 cells/well
(passage 3) were seeded in a 6-well plate. After 24
hours, the proliferative medium was replaced with
adipogenic differentiation medium [DMEM (low
glucose) supplemented with 10-7 M dexamethasone,
66 nM insulin, 0.2 mM indomethacin and 0.5 mM
isobutylmethylxanthine (Sigma-Aldrich, St. Louis,
Mo, USA)]. The cells were incubated at 37°C and
5% CO2. After 14 days, the cells were fixed with 3%
paraformaldehyde and the presence of lipid follicles
was examined by Oil Red O staining (0.5% in methanol,
Sigma-Aldrich, St. Louis, Mo, USA) (22, 24).
Bromodeoxyuridine labeling of adipose tissue-derived
mesenchymal stem cells
For labeling the AT-MSCs prior to transplantation
we used Bromodeoxyuridine (BrdU), which is a base
analogue substituted for thymine during DNAsynthesis
in proliferating cells. Following the denaturation
of double-stranded DNA, BrdU is detected by
immunohistochemistry, thus a population of cells that
has proliferated is identified (25). Using this method
we were able to trace the transplanted cells in the
murine testicles. To do so, passage 3 AT-MSCs were
incubated in 10 mM BrdU (Sigma-Aldrich, St. Louis,
Mo, USA) overnight and BrdU immunohistochemistry
kit (Merck, Germany) was used to confirm labeling of
the cells.
Induction of azoospermia by surgical testicular
torsion-detorsion procedure
To create azoospermic mice, we used the testicular
torsion-detorsion method. For this purpose, twenty
6-8 week-old male NMRI mice (25-30 g) were first
anesthetized by intraperitoneal injection of ketamine
and xylazine, then the scrotal midline was cut, tunica
vaginalis was opened and the testicle was twisted 720
degrees around its axis in a counterclockwise direction
and was fixed with a 4-0 silk suture. Two hours later (26),
the testicle was untwisted and fixed to the scrotal wall,
which was then surgically closed (27). The right testicle
of each group was also considered as the positive control
for that group.
Six weeks after testicular torsion-detorsion surgery,
the mice were anesthetized with ketamine/xylazine,
scrotal walls were opened and 105 AT-MSCs were
injected into the lumen of seminiferous tubules of
testicular torsion-detorsion mice by Hamilton syringes.
Testicles were fixed in their places and scrotal walls
were closed again. The mice were divided into three
groups. Group 1 was injected with AT-MSCs cultured
in EGF (10 ng/ml), LIF (5 ng/ml), and GDNF (5 ng/
ml) (MSCs-GF group), group 2 was injected with AT-
MSCs that were cultured in a medium without growth
factors (MSCs-T group), and group 3 was the testicular
torsion-detorsion mice that did not receive any cells
(negative control). The right testicles of all mice were
considered as the positive control group for each
treatment. To verify that the injected AT-MSCs have
entered the testicles, the cells were stained with trypan
blue. 8 weeks after cell transplantation, 5 testicles in
each group were removed for molecular analysis. For
histological analyses, 3 testicles in each group were
removed and fixed in formalin and hematoxylin-eosin
staining and immunohistochemical analysis were
performed on tissue sections.
Hematoxylin-eosin staining
For histological assessment, hematoxylin-eosin staining
was done. The stages of staining were performed according
to the standard protocols, as summarized in the study by
Cardiff et al. (28). All reagents were from Sigma-Aldrich
(St. Louis, Mo, USA).
Immunohistochemical assessments of testicles
In order to trace the AT-MSCs labeled with BrdU,
immunohistochemical staining was performed. For
this purpose, the tissues containing BrdU were fixed
in 4% formalin, then dehydrated and embedded in
paraffin. Five-micron thick slices were prepared
from the paraffin blocks and placed on slides for
immunostaining. The slides were kept at 37°C
overnight. Prior to staining, the sections were
deparaffinized, then staining was performed according
to the BrdU immunohistochemistry kit (Merck,
Germany) instructions.
RNA extraction, cDNA synthesis and real time
polymerase chain reaction
The RNeasy Mini Kit (Qiagen, Germany) was used
to extract the total tissue RNA as per the company
instructions. The cDNA was synthesized with Quanti
Nova Reverse Transcription Kit (Qiagen, Germany)
according to the company instructions. Primers for the
selected genes were designed specifically using Gene
Bank sequences. Primer sequences of c-Kit, Mvh,
Scp3, Gcnf and Gapdh are as follows respectively:F: 5´-GAGAAGGAAGCGTGACTCGT-3´R: 5´-TCTTGCGGATCTCCTCTTGT-3´,F: 5´-CGAAACATAGGTGATGAAAGAAC-3´R: 5´-CCACTGAAGTAGCAACAAGAAC-3´,F: 5´-AAAGCATTCTGGGAAATCTG-3´R: 5´-GTACTTCACCTCCAACATCTTC-3´,F: 5´-CAACTGAACAAGCGGTATT-3´R: 5´-GATGTATCGGATCTCTGGC-3´,F: 5´-AAGGTCATCCCAGAGCTGAA-3´R: 5´-CTGCTTCACCACCTTCTTGA-3´.Quantitative real-time polymerase chain reaction
(qRT-PCR) stages were performed in Applied
Biosystems 7500 Sequence Biosystem. Briefly, 100
nM of the primers and 100 ng cDNA were added to
Syber Green PCR master mix to reach the overall
volume of 10 µl, then the reaction was carried out in
45 cycles, at 95°C for 15 seconds and 58-60°C for 1
minutes. The gene expression levels in every sample
were normalized with the Gapdh gene and data was
evaluated using 2-ΔΔCT approach (22).
Western blot analysis
To assess the expression of c-Kit and Gcnf proteins,
western blot analysis was performed. In this method,
tissue samples were lysed in radioimmunoprecipitation
assay buffer (RIPA) solution [150 mM NaCl, 25 mM
Tris-HCl (pH=7.6), 1% Triton X-100, and, 1 mM EDTA
pH=7.4, 3% sodium dodecyl sulfate (SDS, Sigma-
Aldrich, St. Louis, Mo, USA), 1% Sodium deoxy
collate] supplemented with 0.1% phosphatase inhibitor
(Sigma-Aldrich, USA). The concentrations of the
proteins was specified using bicinchoninic acid assay
(BCA assay). The equivalent quantity of the protein
samples (60 µg) was loaded on 12% polyacrylamide
gel, and then transferred to polyvinylidene fluoride
(PVDF) membrane (Amersham, UK). PVDF membrane
was blocked at room temperature for one hour in Tris
Buffer/Tween 20 (TBST) solution containing 3% skim
milk. Then, the membrane was incubated with primary
antibodies in the blocking buffer at 4°C overnight: Gcnf
(1:1000, Abcam, USA), c-Kit (1:250, Abcam, USA),
ß-actin (1:250, Santa Cruz Biotechnology, Germany).
After washing with TBST, the membrane was exposed
to the secondary antibody in the blocking buffer [goat
anti rabbit IgG-HRP (1:15000, Abcam, USA)] for one
hour at room temperature. The membrane was then
washed in TBST and enhanced chemiluminescence
(ECL) western blotting substrate (Abcam, USA) was
used for detection of the protein bands according to
the manufacturer’s instructions. Beta-actin protein
was used as a loading control. Image J software was
used to measure and compare the density of the protein
bands in the experimental and control groups.
Statistical analysis
For the analysis of the real time PCR tests, the relative
expression levels of the genes were calculated by the 2-..CT
formula and SPSS version 16 (SPSS Ink,. USA) was used
for statistical analysis. All quantitative variables were
expressed as mean ± SD. The variations were evaluated
using one way analysis of variance (ANOVA), Kruskal-
Wallis test, Dunnett test and LSD test. For all statistical
analyses, the statistical significance was set as P=0.05.
AT-MSCs were isolated from the adipose tissue
around epididymis of male NMRI mice as was
explained before. On the first day, the isolated cells
were round shaped, but three days later, the cells
became spindle-shaped and fibroblast-like. Other
types of cells including endothelial and blood cells
were also seen in the flask, however, these cells were
eliminated during passaging (Fig .1).
Fig.1
Morphology of the cultured adipose tissue derived mesenchymal stem cells. A. Day 0, B. Day 3, C. Day 5, and D. Passage 1 (scale bar: 100 µm).
Morphology of the cultured adipose tissue derived mesenchymal stem cells. A. Day 0, B. Day 3, C. Day 5, and D. Passage 1 (scale bar: 100 µm).Nine days after the induction of adipogenic differentiation,
lipid vacuoles within the cells were observed. After 14
days, the cells were stained with Oil Red O and the lipid
particles turned red (Fig .2A). The first signs of change in the
morphology of AT-MSCs and differentiation to osteocyte cells
were seen 10 days after inducing osteogenic differentiation.
After 21 days, the cells started forming calcium nodules. The
cells formed mineral matrixes around themselves that were
visible by Alizarin Red staining (Fig .2B). The results showed
that these cells have the potentials to differentiate into both
adipogenic and osteogenic lineages.
Fig.2
Adipose tissue derived mesenchymal stem cells exhibited stem
cell characteristics. A. Adipocyte differentiation of the cells. Arrows showlipid vacuoles stained with oil red O and B. Differentiation of the cells into
osteocytes. The arrows show the calcium nodules stained with alizarin red(scale bar: 100 µm).
According to the results of our previous study, the isolatedcells expressed high levels of CD90 and CD44 markers, andshowed low expressions of CD31 and CD45. These values
indicated a high level of purity of the isolated MSCs (22).Adipose tissue derived mesenchymal stem cells exhibited stem
cell characteristics. A. Adipocyte differentiation of the cells. Arrows showlipid vacuoles stained with oil red O and B. Differentiation of the cells into
osteocytes. The arrows show the calcium nodules stained with alizarin red(scale bar: 100 µm).
Histological analysis of recipient mice testis
Six weeks after torsion-detorsion surgery of mice,
hematoxylin-eosin staining of testicle tissue sections was
performed. In the seminiferous tubules of the testicular
torsion-detorsion mice, most of the sperm cells were
eliminated, spermatogenesis was arrested and the tubules
were empty from spermatogenic cells, while Sertoli cells and
seminiferous tubules structures were maintained (Fig .3). Eight
weeks after cell transplantation, most of the labeled cells had
survived and were resided in the basement membrane of the
seminiferous tubules. Spermatogenesis process successfully
occurred in seminiferous tubules and spermatogenic cells
were observed in these tubules (Fig .4).
Fig.3
H&E staining of testis sections. A. Positive control (scale bar: 50
µm), B. Torsion testis: six weeks after the torsion/detorsion, most of
sperm cells were eliminated, and C. Cell transplanted testis after 8 weeks,
spermatogenesis was observed in seminiferous tubules (scale bar: 100 µm).
Fig.4
Bromodeoxyuridine (BrdU) staining of the cells and tissues. A. The labeled cells with BrdU before transplantation. Arrows show the labeled cells,
B. Positive control, intestinal mouse cells, C, and D. BrdU labeled cells transplanted into mouse testis. Most of the cells were localized into the basement
membrane of seminiferous tubules (the brown cells in C and the dark cells in D). BrdU-labeled cells are shown by arrows (scale bar: 50 µm).
H&E staining of testis sections. A. Positive control (scale bar: 50
µm), B. Torsion testis: six weeks after the torsion/detorsion, most of
sperm cells were eliminated, and C. Cell transplanted testis after 8 weeks,
spermatogenesis was observed in seminiferous tubules (scale bar: 100 µm).
Expression of spermatogenic molecular markers in
testicle of transplanted mice
The expression levels of Gcnf gene, a germ cell-specificmarker, in both MSCs-GF (P<0.001) and MSCs-T groups(P<0.01) increased significantly compared to the control
group. Gcnf gene expression in the MSCs-GF group wassignificantly higher than that in MSCs-T group (P<0.001).
The expression level of Mvh another germ cell-specificmarker, in the MSCs-GF group was significantly highercompared to the control group (P<0.05). The expression ofthis gene was not significantly different in the MSCs-T group.
The expression levels of Scp3 and c-Kit markers showed no
significant difference in either experimental group compared
to the control group (Fig .5).
Fig.5
Expression of spermatogenic molecular markers in testicle of the transplanted mice. A. The Gcnf expression in MSCs-GF group (P<0.001) and MSCs-T
group (P<0.01) increased compared to the control group, B. The expression of Mvh, in the MSCs-GF group showed a significantly higher level than the
control group (P<0.05), C, and D. Expression of Scp3 and c-Kit markers showed no significant difference compared to the control group. *; P<0.05, **;
P<0.01, ***; P<0.001, MSCs; Mesenchymal stem cells, AT-MSCs; Adipose tissue-derived MSCs, MSCs-T; The group of mice injected with AT-MSCs, and
MSCs-GF; The group of mice injected with AT-MSCs cultured with growth factors, torsion: negative control.
Bromodeoxyuridine (BrdU) staining of the cells and tissues. A. The labeled cells with BrdU before transplantation. Arrows show the labeled cells,
B. Positive control, intestinal mouse cells, C, and D. BrdU labeled cells transplanted into mouse testis. Most of the cells were localized into the basement
membrane of seminiferous tubules (the brown cells in C and the dark cells in D). BrdU-labeled cells are shown by arrows (scale bar: 50 µm).Expression of spermatogenic molecular markers in testicle of the transplanted mice. A. The Gcnf expression in MSCs-GF group (P<0.001) and MSCs-T
group (P<0.01) increased compared to the control group, B. The expression of Mvh, in the MSCs-GF group showed a significantly higher level than the
control group (P<0.05), C, and D. Expression of Scp3 and c-Kit markers showed no significant difference compared to the control group. *; P<0.05, **;
P<0.01, ***; P<0.001, MSCs; Mesenchymal stem cells, AT-MSCs; Adipose tissue-derived MSCs, MSCs-T; The group of mice injected with AT-MSCs, and
MSCs-GF; The group of mice injected with AT-MSCs cultured with growth factors, torsion: negative control.
Protein analysis after adipose tissue-derived
mesenchymal stem cell transplantation
c-Kit protein expression in both MSCs-GF and
MSCs-T groups showed no difference compared to the
control groups and confirmed the results of the real time
PCR method. Expression of Gcnf protein in the MSCs-
GF group was higher than the control group (P<0.05),
but the MSCs-T group showed no significant difference
compared to the control group (Fig .6).
Fig.6
Western blot results. A, B. c-Kit protein expression results (not
statistically significant), C, and D. Expression of Gcnf protein in the
MSCs-GF group was higher but the MSCs-T group showed no significant
difference compared to the control group. *; P<0.05, MSCs; Mesenchymal
stem cells, AT-MSCs; Adipose tissue-derived MSCs, MSCs-T; The group
of mice that received AT-MSCs, and MSCs-GF; The group of mice that
received AT-MSCs cultured with growth factors, torsion: negative control.
Western blot results. A, B. c-Kit protein expression results (not
statistically significant), C, and D. Expression of Gcnf protein in the
MSCs-GF group was higher but the MSCs-T group showed no significant
difference compared to the control group. *; P<0.05, MSCs; Mesenchymal
stem cells, AT-MSCs; Adipose tissue-derived MSCs, MSCs-T; The group
of mice that received AT-MSCs, and MSCs-GF; The group of mice that
received AT-MSCs cultured with growth factors, torsion: negative control.
Discussion
Stem cell-based therapy has become one of the new
potential treatment for the near future in regenerative
medicine for the repair of damaged tissues and organs in
many diseases such as infertility (29). AT-MSCs can be
obtained easily and are highly capable of proliferation and
differentiation into different lineages. These fibroblast-
like cells have high immune-modulating properties.
Therefore, they are considered appropriate options for
autologous cell transplantation (30).Most of the previous studies show that MSCs confer
potential of spermatogenesis recovery in azoospermic
animal models (5, 31-33). Nayernia et al. (9) was the first
group who reported that murine (BM)-MSCs possess
a high differentiating potential into male germ cells.
Zhang et al. (10) demonstrated that BM-MSCs have the
capability of differentiating into sperm-like cells and
restoring fertility in busulfan treated azoospermic rats
Ghasemzadeh- Hasankolaei’s group (34) as well as Anand
et al. (35) have also reported similar results. Vahdati et al.
(32) have shown that BM-MSCs revive spermatogenesis
of infertile hamsters. Consistent with our results, Cakici
et al. (11) also showed the restoration of the fertility of
azoospermic rats after injection of AT-MSCs. Hsiao et al.
(33) have reported that through inhibition of apoptosis
and enhancement of testosterone secretion, MSCs prevent
infertility in torsion rats. These findings indicate that
MSCs successfully differentiate into germ cells in animal
models and have the potentials to be used in the treatment
of infertility in human patients as well.In the present study, one group of mice was injected with
AT-MSCs cultured in a medium supplemented with EGF,
LIF, and GDNF growth factors. These factors increase
proliferation and viability of the AT-MSCs in vitro (22).
They are also secreted in the testicular niche that influences
the proliferation process and maintenance of SSCs (17,
21). Spermatogenesis process occurs in seminiferous
tubules. The core components of testicular niche include
the basement membrane, Sertoli cells, peritubular myoid
cells, and the extracellular signaling molecules. Sertoli
cells are one of the most important of these components
and provide the necessary growth factors for proliferation
and maintenance of SSCs (36). We injected the cells
into the semniferous tubules of azoospermic mice. In
fact, an appropriate microenvironment was provided for
differentiation of MSCs. In previous studies, a busulfantreated
azoospermic mouse model was used as recipient
(10, 11). One limitation of using this model is damaging
seminiferous tubules structure and destroying the
testicular niche, especially Sertoli cells through busulfan
treatment.Transplanted AT-MSCs migrate to the basement
membrane of seminiferous tubules. They are affected
by the seminiferous tubules niche and factors secreted
by Sertoli cells, and begin to differentiate. In studies
conducted by Zhang et al. (10) and Cakici et al. (11),
a small number of the cells remained in the basement
membrane after injection. However, in our study, after 8
weeks, a large number of AT-MSCs were resided in the
seminiferous tubules basement membrane, which can be
due to the increase of viability of the cells induced by the
growth factors as well as an appropriate mouse model, in
which the structure of seminiferous tubules and testicular
niche have been maintained.After 8 weeks, Gcnf gene expression in the cell-
transplanted groups (MSCs-GF and MSCs-T) was
significantly higher compared to the control group.
Interestingly, MSCs-GF group showed further increased
expression of the germ cell-specific markers (Mvh, Gcnf).
It could be due to the impact of the growth factors on
viability of the cells. In addition, EGF, LIF, and GDNF
are secreted from sertoli cells and testicular niches (17,
21). Therefore, they are probably effective in the process
of differentiation of the injected cells into germ cells.
Expression of c-Kit and Scp3 genes in the AT-MSC
recipient groups did not significantly differ from the
control group. These genes are related to the final stages
of sperm differentiation (37). However, this could be
due to our short tracking time. Zhang et al. (10) showed
increased expression of Mvh and Gcnf factors in the
testicular tissues and reported that c-Kit expression was
reduced after 8 weeks. The exact mechanism of function
of the transplanted MSCs has not been specified. There
are several possibilities in this regard: i. MSCs are
differentiated into target tissue cells under the influence
of their niche (38), ii. MSCs secrete factors, which
stimulate inner stem cells or lead to revival of damaged
tissue (7), and iii. In the case of infertility, MSCs can
prevent infertility by inhibition of oxidative stress and
apoptosis (33).The observations in the present study may indicate
that the injected AT-MSCs have entered spermatogenic
pathway or have revived damaged testicular tissue and
SSCs by secretion of trophic factors. To determine its
exact mechanism, the cells should be tracked over a
longer period of time in the future studies.
Conclusion
This study showed that the transplanted AT-MSCs were
localized in the basement membrane of seminiferous
tubules. The testicles of the mice injected with AT-MSCs
expressed spermatogenesis-specific markers. The mice
that received cells that were cultured in the presence
of growth factors showed overexpression of germ cell-
specific markers. According to these results, the use of
EGF, LIF and, GDNF to culture AT-MSCs can be very
helpful in terms of MSC survival and localization, but
further preclinical studies in different animal models
and with different time points are needed to develop an
effective clinical application.
Authors: Ali Cay; Ahmet Alver; Murat Küçük; Osman Işik; M Selçuk Eminağaoğlu; S Caner Karahan; Orhan Değer Journal: J Surg Res Date: 2006-01-18 Impact factor: 2.192
Authors: Karim Nayernia; Jessica Nolte; Hans W Michelmann; Jae Ho Lee; Kristina Rathsack; Nadja Drusenheimer; Arvind Dev; Gerald Wulf; Ingrid E Ehrmann; David J Elliott; Vera Okpanyi; Ulrich Zechner; Thomas Haaf; Andreas Meinhardt; Wolfgang Engel Journal: Dev Cell Date: 2006-07 Impact factor: 12.270
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