Ebrahim Cheraghi1, Alireza Golkar2, Kambiz Roshanaei3, Behrang Alani4. 1. Department of Biology, Faculty of Sciences, University of Qom, Qom, Iran. Electronic address: e.cheraghi@qom.ac.ir. 2. Sciences Research Laboratory, Department of Biology, Qom Branch, Islamic Azad University, Qom, Iran. 3. Department of Biology, Qom Branch, Islamic Azad University, Qom, Iran. 4. Department of Applied Cell Sciences, Faculty of Medicine, Kashan University of Medical Sciences, Kashan, Iran.
Aluminum (Al) is the most common metallic element
and the third most common element in the
Earth’s crust (1). The ionic form of this metal is
detectable not only in all natural waters, but also
most types of animal and plant tissues. Due to its reactivity, Al is naturally found in combination
with other elements to form compounds such as
Al sulfate and chloride (2). Al compounds are extensively
used in a wide range of products from
household cookware and storage utensils to water
purification agents, pharmaceuticals (such as
antacids, vaccines, anti-diarrhea drugs, phosphate
binders, and allergy immunotherapy injections),
food additives, and even toothpastes (3).The great abundance of Al increases the risk of
exposure and related health issues in humans (4).
High consumption of Al-containing products will
increase the concentration of this metallic element
in the consumers’ organs and damage their various
tissues (including the testicular tissues of humans
and animals). Moreover, high levels of Al in spermatozoa
and seminal plasma of humans have been
reported to reduce sperm viability and motility (5,
6). Krasovskiĭ et al. (7) have confirmed the gonadal
toxicity of lead and Al chloride in guinea pigs and
rats. Guo et al. (8) have attributed the oxidative
damage and testicular toxicity caused by Al to the
reduction in testis acetyl cholinesterase (AChE) activity.
Chinoy et al. (9) have also found the 30-day
consumption of sodium fluoride and Al chloride to
cause structural changes in the testis, such as formation
of giant cells. Testicular Al accumulation,
necrosis of spermatocytes/spermatids, and a significant
reduction in fertility were also observed in
both male rats and mice (10, 11). Al may cause male
reproductive toxicity through various mechanisms
such as inducing oxidative stress, interfering with
spermatogenesis and steroidogenesis, impairing
cell signaling, disrupting the blood-testis barrier,
and affecting the endocrine system (12).In recent years, increasing attention has been
paid to the application of nutritional antioxidants
(such as herbal products) in diseases related to oxidative
stress. The protective effects of herbal products
have been attributed to their role as free radical
scavengers and antioxidant defense regulators
(13). Curcumin (Curcuma longa Lin, CUR), such
as the active component of turmeric, can serve as
an antioxidant and therapeutic agent without any
side effects (14). As a free radical scavenger, CUR
can largely inhibit the production of reactive oxygen
species (ROS) both in vitro and in vivo. It also
exhibits anti-carcinogenic, anti-inflammatory, and
antibacterial properties (15), as well as acts a potent
cancer chemopreventive agent (16) and tumor
cell proliferation inhibitor (17).Despite the reported antioxidant properties of
CUR (18-21), its effects on apoptosis, oxidative
stress and sperm quality in Al-treated rats have
not been investigated. Therefore, the present study
analyzed the protective effects of CUR on Al-induced
damage to the reproductive system of male
rats.
Materials and Methods
CUR powder (C21H20O6, Merck & Co. Inc.,
Germany) was dissolved in dimethyl sulfoxide
(DMSO). Al chloride (Merck & Co. Inc., Germany)
was diluted with distilled water before administration.
Experimental protocol
In this experimental study, a total of 40 male
Wistar rats (240-260 g) were obtained from
the animal house of Razi Institute (Iran). Rats
were housed in individually ventilated cages
on a 12-hour light/dark cycle, temperature of
24 ± 2ºC, with water and food ad libitum. The
experimental protocol was approved by the
Animal Ethics Committee in accordance with
the Guide for the Care and Use of Laboratory
Animals prepared by Qom University of Medical
Sciences (Qom, Iran).Over a two-week adaptation period, all rats were
fed by a standard pellet diet and closely monitored
to ensure normal growth and behavior. The rats
were then weighed and randomly allocated to five
groups of eight animals (two control groups and
three experimental groups) to receive the following
treatments for 28 days (22, 23): group I (control
group): no injections. Group II (control group):
intraperitoneal (IP) injections of only the solvent
(distilled water or DMSO). Based on the solvents,
we chose two control groups, distilled water and
DMSO. Since there were no significant solvents,
between the results of the control groups, we considered
data from the distilled water group as the
control group. Group III (experimental group): IP
injections of CUR 10 mg/kg body weight (BW)
(22) in 0.2 ml DMSO. Group IV (experimental
group): IP injections of Al chloride 10 mg/kg BW
(23) in 0.2 ml distilled water. Group V (experimental
group): IP injections of CUR+Al chloride
at the above-mentioned doses alone.All groups were fed by a normal diet. After the
treatment period, the rats were reweighed that was
followed by being euthanized and dissected. Blood
samples were collected into heparinized capillary
tubes through cardiac puncture. In order to
separate the plasma, the samples were poured into
clean tubes and centrifuged at 1500 g for 20 minutes
at 4°C. Testis and epididymis were detached
from the adhering connective tissues, washed in
cold physiological saline, and weighed accurately.
Plasma hormone assay
Plasma was obtained and maintained at -20°C
until enzyme-linked immunosorbent assay (ELISA)
was performed. The concentrations of luteinizing
hormone (LH), follicle-stimulating hormone
(FSH) and testosterone were determined using
ELISA kits (Elabscience Biotechnology Co., Ltd.,
Germany) according to the manufacturer's instructions.
All measurements were carried out in duplicate.
The intra- and inter- assay coefficients of
variation were less than 10%.
Assessment of lipid peroxidation
Thiobarbituric acid reactive substance (TBARS)
levels were determined as a measure of plasma
concentrations of malondialdehyde (MDA), the
end product of lipid peroxidation (LPO) (24).
MDA levels were reported as nmol/ml.
Assessment of superoxide dismutase levels
Superoxide dismutase (SOD) activity in plasma
was measured using a commercial assay kit (Cayman
Chemical, USA) according to the manufacturer's
instructions. This kit utilized a tetrazolium salt
for the detection of superoxide radicals generated
by xanthine oxidase and hypoxanthine. One unit of
SOD was defined as the amount of enzyme needed
to exhibit 50% dismutation of the superoxide radical.
The SOD assay measured all three types of
SOD (Cu/Zn, Mn, and Fe SOD) in U/ml (25).
Sperm parameters
Assessment of sperm motility and count
The right cauda epididymis was incised and
semen was pressed on a pre-warmed slide. Two
drops of warm 2.9% sodium citrate were added to
semen and mixed with a coverslip. The percentage of sperm motility was evaluated visually (magnification:
×40). Motility estimates were performed
from three different fields in each sample. The
mean of the three successive estimations was used
as the final motility score. For sperm count, the left
cauda epididymis was incised and the dripped semen
was quickly sucked into a red blood pipette
to the 0.5 mark. The collected semen was diluted
with warm normal saline up to the 101 mark.
Approximately 10 μL of the semen mixture was
placed on a Neubauer chamber and viewed (magnification:
×40). The total numbers of sperm cells
were counted and expressed as 106/ml (26).
Assessment of sperm viability and morphology
Eosin/nigrosin staining was used to determine
sperm viability (percentage of live spermatozoa).
A drop of semen (50 μL) with two drops of the
stain (100 μL) was placed on a microscope slide.
Thin smears were then prepared and observed
under a light microscope (magnification: ×100).
While viable sperms remained colorless, nonviable
sperms appeared red. The stained and unstained
sperm cells were counted. The mean values
for each group were then recorded and used
in percentage viability calculation. In order to determine
the percentage of morphologically abnormal
spermatozoa, eosin-nigrosin staining was performed,
and the slides were viewed under a light
microscope (magnification: ×100). A total of 200
sperm cells were examined on each slide, and the
head, tail and total abnormality rates of spermatozoa
were expressed as a percentage (27).
Histological analysis
In brief, an abdominal incision was made, while the
testes were carefully dissected and fixed in 10% formal-
saline. After paraffin embedding, the sections of 5
μm thickness were obtained using a rotary microtome,
stained with Heidenhain’s Azan, and observed under a
light microscope (magnification: ×200) (28).
TUNEL method for analysis of apoptosis
The in-situ DNA fragmentation was visualized by
terminal deoxynucleotidyl transferase dUTP nick
end labeling (TUNEL) method. Briefly, dewaxed
testis sections were predigested with 20 mg/ml
proteinase K for 20 minutes and incubated in phosphate
buffered saline (PBS) solution containing 3% H2O2 for 10 minutes to block the endogenous peroxidase
activity. The sections were incubated with
the TUNEL reaction mixture, fluorescein-d UTP
(Roche Applied Science, Germany), for 60 minutes
at 37°C, according to the manufacturer’s instructions.
The slides were then rinsed three times with
PBS and incubated with secondary anti-fluorescein-
POD-conjugate for 30 minutes. After washing three
times in PBS, Hoechst stain (Sigma-Aldrich, USA)
was added for chromogenic reaction. As a control
for method specificity, the step using the TUNEL
reaction mixture was omitted in negative control
serial sections, so nucleotide mixture in reaction
buffer was used instead. The apoptotic index was
determined at 10-random locations within each
seminiferous tubule. In all groups, 100 seminiferous
tubules for each animal were recorded (29).
Statistical analysis
The normality of continuous variables was confirmed
using the Kolmogorov-Smirnov test. Data
were reported as mean ± SE and analyzed with oneway
analysis of variance (ANOVA) and Tukey’s
test for post-hoc analysis. P<0.05 were considered
significant. All analyses were performed with the
Statistical Package for the Social (SPSS) for Windows
16.0 (SPSS Inc., USA).
Results
Effects of curcumin and aluminum on sperm
characteristics, the testis and body weight
Significant reductions in sperm count (P=0.0001),
motility (P=0.0001), viability (P=0.001), and morphology
(P=0.001) were detected in rats treated
with Al chloride compared to control group.
Moreover, sperm parameters were significantly higher in rats treated with CUR alone (P=0.0001)
compared to those treated with Al chloride, but
this value was the same in control group (P>0.05).
Rats treated with CUR+Al chloride had significantly
higher sperm count (P=0.001), motility
(P=0.006), viability (P=0.001), and morphology
(P=0.001) compared to Al-treated rats (Table 1,
Figes.1, 2). As Table 1 shows, while the testis and
body weights were significantly reduced in Altreated
rats (P=0.001) compared to control group,
the values were similar in other groups (P>0.05).
Table 1
Changes in body weight, testis weight, sperm count, sperm motility, sperm viability and sperm abnormalities in experimental groups
Parameter
Experimental group
Control
Solvent
CUR
Al
CUR+Al
Body weight (g)
276.1 ± 3.1a
279.6 ± 3.8a
284.4 ± 5.1a
245.2 ± 4.2b
280.6 ± 5.4a
Testis weight (g)
1.36 ± 0.04a
1.35 ± 0.05a
1.37 ± 0.03a
1.09 ± 0.02b
1.34 ± 0.04a
Sperm count (106/ml)
36.22 ± 2.8ac
36.02 ± 3.5ac
45.4 ± 3.5a
17.5 ± 1.1b
32.6 ± 1.9c
Sperm motility (%)
84.8 ± 1.7ac
82.3 ± 3.1ac
87.1 ± 1.7a
43.9 ± 3.8b
68.3 ± 6.3c
Sperm abnormalities (%)
12.34 ± 1.5ac
12.5 ± 1.4ac
9.5 ± 0.7a
40.1 ± 3.2b
20.4 ± 2.8c
Sperm viability (%)
79.8 ± 2.4a
78.5 ± 2.7a
88.9 ± 1.9a
36.3 ± 3.2b
60.7 ± 2.7c
Data are shown as mean ± SE. Means within the same row with different letters are significantly differed (P<0.05) using ANOVA, Tukey's test. CUR; Curcumin and
Al; Aluminum.
Fig.1
Assessment of sperm viability in rats treated by eosin-nigrosin
stain (magnification: ×1000).
A. Alive sperm and B. Dead sperm.
Fig.2
Some of abnormal sperm tail and head morphology after
aluminum exposure by eosin-nigrosin stain (magnification:
×1000). A. Amorphous head, B. Cytoplasmic droplet, C. Amorphous
mid-piece and tail, and D. Coiled or curled tail.
Assessment of sperm viability in rats treated by eosin-nigrosin
stain (magnification: ×1000).A. Alive sperm and B. Dead sperm.Changes in body weight, testis weight, sperm count, sperm motility, sperm viability and sperm abnormalities in experimental groupsData are shown as mean ± SE. Means within the same row with different letters are significantly differed (P<0.05) using ANOVA, Tukey's test. CUR; Curcumin and
Al; Aluminum.
Effect of curcumin and aluminum on reproductive
hormones
We observed that testosterone and LH levels
were significantly lower in Al-treated rats compared
to other groups (P=0.01). Testosterone and
LH levels were higher in CUR-treated group than
all other groups. LH and testosterone levels in
CUR+Al treated group were significantly (P=0.04)
different from Al-treated group, but this value was
not significantly different compared to control and
CUR-treated rats (P>0.05, Table 2). There was also
no significant differences in FSH levels among the
five groups (P>0.05).
Table 2
The changes of FSH, LH, Testosterone, MDA and SOD levels in experimental groups
Parameter
Experimental group
Control
Solvent
CUR
Al
CUR+Al
FSH (IU/L)
2.33 ± 0.4a
2.35 ± 0.3a
2.3 ± 0.4a
2.7 ± 0.6a
2.13 ± 0.2a
LH (IU/L)
2.3 ± 0.42a
2.6 ± 0.4a
2.8 ± 0.45a
0.73 ± 0.07b
2.2 ± 0.3a
T (ng/ml)
3.7 ± 0.6a
3.6 ± 0.7a
4.1 ± 0.5a
1.3 ± 0.3b
3.6 ± 0.7a
MDA (nmol/ml)
4.8 ± 0.44a
5.01 ± 0.43a
4.1 ± 0.53a
7.4 ± 0.65b
5.16 ± 0.54a
SOD (U/ml)
8.26 ± 0.4a
8.27 ± 0.33a
8.93 ± 0.43a
3.26 ± 0.42b
7.5 ± 0.43a
Data are shown as mean ± SE. Means within the same row with different letters are significantly differed (P<0.05) using ANOVA, Tukey’s test. CUR; Curcumin, Al;
Aluminum, FSH; Follicle stimulating hormone, LH; Luteinizing hormone, T; Testosterone, MDA; Malondialdehyde, and SOD; Superoxide dismutase.
Effects of curcumin and aluminum on lipid peroxidation
status
Rats treated with Al chloride in comparison with
other groups showed significantly increased MDA
levels (P=0.01) and significantly decreased SOD
activity (P=0.0001). Treatment with CUR+Al
chloride resulted in significant improvement of
LPO status when compared with Al-treated rats (P=0.001), but this value was not significantly different
compared to control and CUR-treated rats
(P>0.05, Table 2).
Effects of curcumin and aluminum on the structure
of the testes
Al chloride treatment led to degeneration and
necrosis with a significant reduction in the diameter
of seminiferous tubules and germinal epithelium
thickness compared to the control group
(P=0.0001). Moreover, the lumen diameter of
tubules was significantly higher in Al-treated
rats than in the control group (P=0.0001). This
effect was milder in rats treated with CUR+Al
chloride, while the values in this group were
close to those in the control group. The diameter
of seminiferous tubules, germinal epithelium
thickness and the lumen diameter of tubules
were similar in CUR-treated rats and control
group (P>0.05, Table 3,Fig .3). In addition, we
observed no significant difference in the nuclear
diameter of spermatogonia among the groups
(P>0.05, Table 3).
Table 3
The changes of histopathology on rat testis in the experimental groups
Parameter
Experimental group
Control
Solvent
CUR
Al
CUR+Al
The diameter of seminiferous tubules (µ)
181.27 ± 0.8a
181.77 ± 0.6a
184.32 ± 1.5a
157.19 ± 1.2b
180.66 ± 1.3a
The lumen diameter of tubules (µ)
77.02 ± 1.5a
77.03 ± 1.4a
74.48 ± 1.45a
98.93 ± 0.73b
78.74 ± 0.82a
The nuclear diameter of spermatogonia (µ)
4.71 ± 0.01a
4.70 ± 0.01a
4.75 ± 0.02a
4.69 ± 0.01a
4.70 ± 0.01a
Germinal epithelium thickness (µ)
56.29 ± 0.4a
55.16 ± 0.8a
57.39 ± 0.6a
36.46 ± 0.6b
51.56 ± 0.9a
Data are shown as mean ± SE. Means within the same row with different letters are significantly differed (P<0.05) using ANOVA, Tukey’s test. CUR; Curcumin and Al;
Aluminum.
Fig.3
Photomicrographs of transverse sections in the testis
(Heiden hain’s azan stain, 5 μm sections, magnification:
×100). A. Testis of control group showing normal histological
structure of seminiferous tubules, B. Testis of aluminum
group showing an increase in the lumen diameter of tubules,
a decrease in the diameter of seminiferous tubules as well as
distorted seminiferous tubules with loss of normal distribution
of epithelial lining and vacuolar cytoplasm (black arrow),
C.Testis of curcumin group showing no histological changes,
and D. Testis of CUR+Al group revealed no histopathological
changes.
The changes of FSH, LH, Testosterone, MDA and SOD levels in experimental groupsData are shown as mean ± SE. Means within the same row with different letters are significantly differed (P<0.05) using ANOVA, Tukey’s test. CUR; Curcumin, Al;
Aluminum, FSH; Follicle stimulating hormone, LH; Luteinizing hormone, T; Testosterone, MDA; Malondialdehyde, and SOD; Superoxide dismutase.The changes of histopathology on rat testis in the experimental groupsData are shown as mean ± SE. Means within the same row with different letters are significantly differed (P<0.05) using ANOVA, Tukey’s test. CUR; Curcumin and Al;
Aluminum.Some of abnormal sperm tail and head morphology after
aluminum exposure by eosin-nigrosin stain (magnification:
×1000). A. Amorphous head, B. Cytoplasmic droplet, C. Amorphous
mid-piece and tail, and D. Coiled or curled tail.Photomicrographs of transverse sections in the testis
(Heiden hain’s azan stain, 5 μm sections, magnification:
×100). A. Testis of control group showing normal histological
structure of seminiferous tubules, B. Testis of aluminum
group showing an increase in the lumen diameter of tubules,
a decrease in the diameter of seminiferous tubules as well as
distorted seminiferous tubules with loss of normal distribution
of epithelial lining and vacuolar cytoplasm (black arrow),
C.Testis of curcumin group showing no histological changes,
and D. Testis of CUR+Al group revealed no histopathological
changes.
Effects of curcumin and aluminum on apoptosis
Rats treated with Al chloride showed significantly
increased TUNEL-positive cells (P=0.001) in comparison
with other groups. Treatment with CUR+Al
chloride resulted in significant increase the number
of TUNEL-positive cells when compared with Altreated
rats(P=0.01, Figes.4, 5). Moreover, the number
of apoptotic cells were significantly decreased
in rats treated with CUR alone (P=0.0001) as compared
to those treated with Al alone and CUR+Al
groups, but this value was not significantly different
compared to control group (P>0.05).
Fig.4
Photomicrograph of the different groups showing the number of apoptotic cells in 100 seminiferous tubules following TUNEL staining.
Values are expressed as mean ± SE (n=8). Values bearing different superscript on the bar diagram vary significantly (P<0.05) using one
way ANOVA and Tukey’s test. Al; Aluminum and CUR; Curcumin.
Fig.5
Effects of CUR and Al on the number of apoptotic cells by fluorescence microscope (magnification: ×400). A. Solvent (control), B.
Treated with Al, C. Treated with CUR, and D. Treated with CUR+Al. Compared with the control group, the number of apoptotic cells were
significantly increased in Al group. The apoptotic of cells (green) can be recognized. Al; Aluminum and CUR; Curcumin.
Photomicrograph of the different groups showing the number of apoptotic cells in 100 seminiferous tubules following TUNEL staining.
Values are expressed as mean ± SE (n=8). Values bearing different superscript on the bar diagram vary significantly (P<0.05) using one
way ANOVA and Tukey’s test. Al; Aluminum and CUR; Curcumin.Effects of CUR and Al on the number of apoptotic cells by fluorescence microscope (magnification: ×400). A. Solvent (control), B.
Treated with Al, C. Treated with CUR, and D. Treated with CUR+Al. Compared with the control group, the number of apoptotic cells were
significantly increased in Al group. The apoptotic of cells (green) can be recognized. Al; Aluminum and CUR; Curcumin.
Discussion
This study evaluated the toxic effects of Al chloride
in male rat and showed that CUR had the capability
to contrary Al toxicity. The present study
confirmed reductions in body and testis weight
following Al exposure. This is similar to previous
research (6). However, the administration of
CUR either alone or in combination with Al chloride
could maintain testis weight at values close to
the control group. This is also in accordance with
previous studies (18, 21, 22). In accordance with
previous findings (30), we observed significantly
lower LH and testosterone levels in the Al-treated
group (compared to the control group). On the
other hand, since LH and testosterone levels were
significantly higher in rats treated with CUR+Al
than in those exposed to Al chloride alone, CUR
could effectively improve sex hormone levels and
decreases the harmful effects of Al. Comparable
findings were also reported by previous research
(31, 32). However, in present study, the FSH values
remained unchanged in all groups. In contrary,
in a study, by Al-Nahari and Al Eisa (33) they
have showed that Al injection was significantly
decreased the rate of FSH. This different is probably
due to the differences in dose and duration of
administration.Al might induce such a reduction in testosterone
levels by blocking calcium channels and hence
down- regulating gonadotrophins secretion in the
hypophysis (34). Al exposure can also suppress
steroidogenesis by increasing testicular nitric oxide
concentrations and decreasing cyclic adenosine
monophosphate (cAMP) (10). Previous studies
showed that Al injection in rat hypocamp was
significantly decreased the rate of glutamate (35).
Probably blocked voltage sensitive calcium cannels
(VSCCs) in cells are responsible for gonadotropin-
releasing hormone (GnRH) synthesis, affecting
calcium influx in those cells, and decreased
the GnRH secretion. Since FSH and LH secretion
is promoted by FSH-releasing hormone (FSHRH)
and LH-releasing hormone (LHRH) factors which
are produced in separated zones in hypothalamus
nucleoli, it is probable that Al inhibited LHRH
production in hypothalamus, but did not effect on
FSHRH production (35). In our study, rate of FSH
was not affected, which may be due to the FSH
synthesis mechanism that is different from LH and
not affected by calcium ion.Based on our findings, Al exposure decreased
sperm quality. Likewise, previous studies documented
reduced sperm count, motility, and viability
following Al treatment (36, 37). Furthermore,
the alteration in antioxidant system, a decrease in
cAMP and an increases in nitric oxide production
caused by Al treatment might have been responsible
for the observed reductions in sperm motility
and viability and increased morphological abnormality
(12). LH stimulates the interstitial cells of
the Leydig to secrete testosterone (34). Therefore,
a reduction in LH and testosterone levels in the
present study, which are critical to spermatogenesis,
following Al exposure can justify the reduced
sperm count in Al-treated rats. In our study, CUR
treatment significantly improved morphological
normality and sperm count, motility, and viability
in rats receiving Al chloride. In other words, CUR
could counteract the negative effects of Al in the
mentioned- reproductive parameters. Comparable
results were reported by Salama and El-Bahr (19),
Sharma and Singh (21), Jalili et al. (22), Al-Nahari
and Al Eisa (33).In agreement with previous research (31), the results
of this study showed that Al increased MDA
level (well-known LPO indicator) and reduced
SOD activity. SOD protects spermatozoa against
spontaneous O2 toxicity and LPO. Several reports
have suggested that AlCl3 may inhibit the activity
of SOD. Since ROS have been indicated to have
a role in steroidogenesis and gametogenesis (12),
the mentioned effects might have been responsible
for the reduced reproductive hormones and poor
sperm quality seen in Al-treated rats. The reduction
in sperm counts and sex organ weights following
Al exposure in the present study can confirm
the role of Al toxicity in increased oxidative stress
and reinforce the role of ROS. Meanwhile, CUR
has been shown to affect several targets in cells for
its biological activity, while it reduced LPO and
enhanced antioxidant levels in rats (13). CUR exhibits
protective effects against oxidative damage
by decreasing the levels of free radicals, through
its free radical scavenging activity, particularly
against oxygen radicals, which inhibit sulfhydryl
(SH)-group oxidation. It inhibits nuclear factor
kappa B (NF-kB) activity, cyclooxygenase-2
(COX-2), and mitogen-activated protein kinase
(MAPK) expression, while it modulates release of
several cytokines and testicular enzyme activities, mRNA expression of 17 β-hydroxysteroid dehydrogenase
(17β-HSD) and cytochrome P450 sidechain
cleavage (CYP450scc) enzyme in steroidogenesis
(13). It seems that CUR raises testosterone
and LH levels and increases the count and motility
of normal sperms in treated groups through enhancing
the anti-oxidant defense by increasing the
expression of anti-oxidant genes in comparison
with Al-treated rats.Al cytotoxicity may be mediated by free radicals
derived from this element and its capability
to induce apoptosis through a wide variety of
mechanisms including production of ROS, LPO,
cell membrane damage, down regulation of Bax
gene expression, diminished activity of alkaline
phosphatase and cAMP reduction in various tissues
(12, 38). In agreement with previous research
(38), the results of this study showed that Al increased
the amount of apoptotic cells compared
with control. However, a number of studies have
suggest that CUR, due to inhibition of NF-κB activation
and cell scattering, can be considered as a
potential therapeutic agent effective against apoptotic
genes to promote cell death and proliferative
processes (39). Assessment of apoptotic cells in
the seminiferous tubules in the testes of rats treated
with CUR+Al showed a significant reduction
in the amount of apoptotic cells compared with Al
group. Comparable results were reported by Aktas
et al. (40). Therefore, we reported that Al induces
oxidative stress and apoptosis in testicular cells,
and that CUR as antioxidant prevents apoptosis
induced by Al.Histopathological analysis in the current study
indicated testicular structures to be different in
Al-treated rats with other groups. In fact, the Altreated
group had thinner germinal epithelium
and very low spermatid and sperm counts in the
lumen. Similar findings have also been reported
by Guo et al. (10) and Kutlubay et al. (41). This
observation could be attributed to the ability of
Al to cause oxidative stress, cross the blood-testis
barrier, promote lipid peroxidation, and ultimately
damage the biological membrane of the testis. The
low sperm count, motility, and viability, as well
as the high morphological abnormality, seen in Altreated
rats confirm the mentioned mechanism. On
the other hand, the protective effect of CUR on the
testis may be demonstrated that it inhibits cellular
damage and apoptosis occurring as a result of oxidative
stress in the spermatogenic cells of seminiferous
tubules and Leydig cells (13). Chandra et al.
(42) have reported CUR to maintain normal serum
testosterone levels and prevent the reduction in
sex organ weights following chromium exposure.
In a study on male Wistar rats, Sharma and Singh
have highlighted the beneficial effects of CUR on
decreasing the reproductive toxicity caused by lindane
(organochlorine pesticide) (21). The protective
effects of CUR have been attributed to its role
in regulating LPO and boosting the antioxidant defense
system. More specifically, CUR significantly
decreased the levels of free radicals (through its
free radical scavenging activity), induced the production
of detoxification enzymes, and provided
protection against degenerative diseases (43). The
findings of the present study suggested that CUR
treatment protected the cellular structure of the
testes by increasing the formation of antioxidant
products and decreasing LPO.
Conclusion
The results of this study highlighted the protective
effects of CUR on male reproductive toxicity
of Al in an experimental rat model. CUR, as powerful
antioxidant, was able to reduce Al-induced
damage and improve sperm quality by decreasing
oxidative stress. We believe that further research
on the utility of CUR may indicate its usefulness
as a potential treatment for spermatogenesis after
testicular injury caused by Al treatment in rats.
Authors: Maha Lokman; Eman Ashraf; Rami B Kassab; Ahmed E Abdel Moneim; Nabil A El-Yamany Journal: Biol Trace Elem Res Date: 2021-11-06 Impact factor: 4.081
Authors: Sadaf Jamal Gilani; May Nasser Bin-Jumah; Fahad A Al-Abbasi; Syed Sarim Imam; Sultan Alshehri; Mohammed M Ghoneim; Muhammad Shahid Nadeem; Muhammad Afzal; Sami I Alzarea; Nadeem Sayyed; Imran Kazmi Journal: ACS Omega Date: 2022-07-01
Authors: Cezary Grochowski; Eliza Blicharska; Jacek Bogucki; Jędrzej Proch; Aleksandra Mierzwińska; Jacek Baj; Jakub Litak; Arkadiusz Podkowiński; Jolanta Flieger; Grzegorz Teresiński; Ryszard Maciejewski; Przemysław Niedzielski; Piotr Rzymski Journal: Molecules Date: 2019-05-03 Impact factor: 4.411
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