Benedict Falana1, Opeyemi Adeleke1, Mulikat Orenolu1, Abraham Osinubi2, Adeoye Oyewopo3. 1. Department of Anatomy, College of Health Sciences, Osun State University, Osogbo, Nigeria. 2. Department of Anatomy, College of Medicine, University of Lagos, Lagos State, Nigeria. 3. Department of Anatomy, College of Health Sciences, University of Ilorin, Ilorin State, Nigeria.
Abstract
OBJECTIVE: This study investigated the effects of D-ribose and L-cysteine on aluminum-induced testicular damage in male Sprague-Dawley rats. METHOD: A total number of thirty-five (35) adult male Sprague-Dawley rats were divided into four groups (AD). Group A (comprised five (5) rats) was designated the Control Group that received Physiological Saline; while groups B, C, and D (comprised ten (10) rats) were given 75 mg/kg, 150 mg/kg and 300 mg/kg of body weight of aluminum chloride respectively for 39 days. At day 40, the aluminum-treated groups were subdivided into sub-groups (B1, C1, D1) comprising of five (5) rats each, and 30 mg/kg body weight of Riboceine were administered for twenty (20) days. Groups B, C and D remained on the normal dosage of aluminum chloride for three more weeks (59 days). RESULTS: Andrological parameters (Sperm count, motility, morphology and testosterone) in the aluminum-treated Groups B and C showed no significant difference in their mean values when compared with their control counterparts, whereas there was a significant reduction in the andrological parameters in Group D rats when compared with the Control animals. Histoarchitecture of the testes "stain with H&E" of Group A, B and C rats appeared normal while Group D rats showed testicular damages with several abnormal seminiferous tubules with incomplete maturation of germinal cell layers and absence of spermatozoa in their lumen; Leydig cells appear hyperplastic. Group B1, C1 and D1 andrological and histological parameters appeared normal. CONCLUSION: Riboceine treatment significantly attenuates aluminum-induced testicular toxicity in male Sprague-Dawley in rats.
OBJECTIVE: This study investigated the effects of D-ribose and L-cysteine on aluminum-induced testicular damage in male Sprague-Dawley rats. METHOD: A total number of thirty-five (35) adult male Sprague-Dawley rats were divided into four groups (AD). Group A (comprised five (5) rats) was designated the Control Group that received Physiological Saline; while groups B, C, and D (comprised ten (10) rats) were given 75 mg/kg, 150 mg/kg and 300 mg/kg of body weight of aluminum chloride respectively for 39 days. At day 40, the aluminum-treated groups were subdivided into sub-groups (B1, C1, D1) comprising of five (5) rats each, and 30 mg/kg body weight of Riboceine were administered for twenty (20) days. Groups B, C and D remained on the normal dosage of aluminum chloride for three more weeks (59 days). RESULTS: Andrological parameters (Sperm count, motility, morphology and testosterone) in the aluminum-treated Groups B and C showed no significant difference in their mean values when compared with their control counterparts, whereas there was a significant reduction in the andrological parameters in Group D rats when compared with the Control animals. Histoarchitecture of the testes "stain with H&E" of Group A, B and C rats appeared normal while Group D rats showed testicular damages with several abnormal seminiferous tubules with incomplete maturation of germinal cell layers and absence of spermatozoa in their lumen; Leydig cells appear hyperplastic. Group B1, C1 and D1 andrological and histological parameters appeared normal. CONCLUSION:Riboceine treatment significantly attenuates aluminum-induced testicular toxicity in male Sprague-Dawley in rats.
Entities:
Keywords:
D-Ribose and L-Cysteine; aluminum chloride; sprague-dawley rats; testes
Mammals', especially human's exposure to metals cannot be overlook. Metals are
ubiquitous and humans can be exposed to it via pollution in the air, water, soil and
food, their wide use in industry and long-term persistence in the environment. Among
these metals is aluminum (Al). Aluminum is the most widely distributed trivalent
cation, which is usually present in plants, animal tissues and in natural water, in
the form of ion. Aluminum prevalence is high when compared to other elements, and
its present in the earth crust is more than enough, representing approximately 8% of
its total mineral components. Aluminum is present in trace amounts in biological
materials and the Agency for Toxic Substances and Disease Registry from the year
2008 reported that aluminum is characterized to have negative effects on general
human health ([ATSDR, 2008]). Al
occurs naturally in the environment, and it is also released due to anthropogenic
activities such as mining and industrial uses, in the production of aluminum metal
and other forms of Al compounds. A variety of Al compounds are produced and used for
different purposes, such as in water treatment, papermaking, fire retardants,
fillers, food additives, pharmaceuticals, colors, cosmetics, Aluminum ware and
containers.Many studies have reported on Aluminum-induced toxic effects in humans or in
laboratory animals. Overexposure to aluminum has been reported to have deleterious
effects on testicular tissues ([Pizent ]). Metals have been shown to affect
spermatogenesis in rodents and humans, which can lead to low sperm count, abnormal
sperm morphology and poor semen quality ([Pizent
]).Experimental studies have suggested that certain mechanisms might be involved in the
male reproductive toxicity of aluminum, and these include impairment of the
blood-testis barrier, histological alterations and increased oxidative stress
([Berihu ]). Oxidative stress reflects an imbalance between the
systemic manifestation of reactive oxygen species and a biological system's ability
to readily detoxify the reactive intermediates or to repair the resulting damage.
Thus, causing disruptions in normal mechanisms of cellular signaling and cell death
([]). One of the biological systems (antioxidants)
that detoxifies reactive oxygen species or that repairs the resulting damages caused
by free radicals is Glutathione. Sometimes these free radicals overpower the
biological systems, thus the body may need external supplements to complement the
production of antioxidants ([]).Riboceine is one of the synthetic antioxidants that help cells produce glutathione
on-demand. The active ingredient of riboceine is D-Ribose-L-Cysteine. Whole
glutathione consumption cannot be effective because it would be destroyed in the
digestion process before reaching the cell. The ribose component of the Riboceine
solves these challenges by effectively protecting and delivering the fragile
cysteine molecule, enabling the cells to produce glutathione when the cells need it
most. Hence, this study is aimed at investigating the oral administration of
Riboceine on Aluminum-induced testicular damage in Sprague-Dawley rats.
MATERIALS AND METHODS
Aluminum Chloride and Riboceine Preparation
Aluminum chloride was procured and prepared in the Department of Biochemistry,
Osun State University, while Riboceine was obtained from the University of
Lagos. The preparation was done by separately dissolving 100 mg of the Aluminum
Chloride and Riboceine in 100 ml of distilled water (1ml of the solution contain
1mg of the solvent).
Experimental Design
A total number of thirty-five (35) adult male Sprague-Dawley rats were divided
into four groups (A-D). Group A (comprised five (5) rats) was designated the
Control group - receiving saline solution, while groups B, C, and D (comprised
ten (10) rats) were given 75 mg/kg, 150 mg/kg and 300 mg/kg body weight of
aluminum chloride, respectively, for 39 days. At day 40, the aluminum-treated
groups were subdivided into sub-groups (B1, C1, D1) comprised of five (5) rats
each and 30 mg/kg body weight of Riboceine were administered for Twenty (20)
days. Groups B, C and D remained on the normal dosage of aluminum chloride for
three weeks more (59 days). The animals were fed with feed from TopFeeds Ltd.
Osogbo, Osun State, Nigeria, with ad libitum access to drinking water. All the
experimental procedures were done following the experimental guidelines of the
Health Research and Ethics Committee (HREC) of the Osun State University, Osogbo
Campus, Osogbo, Osun State.
Animal Slaughter and Samples Collection
The animals were slaughtered on the sixtieth (60th) day of the
experiment, being anaesthetized with 0.5ml/kg of ketamine hydrochloride and
fixed by transcardial perfusion method using 4% paraformaldehyde as fixative
agent. Caudal epididymis was excised from the testes prior to perfusion fixation
for sperm analysis and the testes were fixed in Bouin's fluid for histological
analysis.
Sperm count assay
Sperm motility was assessed by the method described by [Rouge & Bowen, 2002]. The spermatozoa were
counted by hemocytometer using the improved Neubauer (Deep 1/10 mm, LABART,
Germany) chamber, as described by [Rouge
& Bowen, 2002].
Sperm morphology and motility assay
Sperm live/dead ratio and motility was determined using 1% Eosin and 5% Nigrosin
in 3% sodium citrate dehydrate solution according to the method described by
[Rouge & Bowen,
2002].
Testosterone assay
This was carried out with the use of the Testosterone ELISA Kit obtained from
Monobind Inc. Lake forest, CA, U.S.A. The essential reagents used for this assay
were biotinylated antibody, enzyme-antigen conjugate and a serum native antigen,
upon mixing all these reagents, a competitive reaction set-in between the native
antigen and enzyme antigen conjugate for a limited number of antibody binding
sites. The amount of testosterone able to bind to the testosterone antiserum
will be inversely proportional to the concentration of testosterone in the well.
The absorbance in each well at 450nm was read in a microplate reader (using a
reference wavelength of 620630nm to minimize well imperfections).
Histological examination
Routine histological processing using Hematoxylin and Eosin staining method was
carried out. The testes were fixed in Boiun's, dehydrated in ascending grades of
alcohol, cleared in xylene, infiltrated in molten paraffin wax before finally
embedded in molten paraffin wax in order to form the paraffin block. The
paraffin block containing the tissue was then sectioned by the rotary microtome
at 4µσι thickness. The sections were then floated in water
bath at 400c and transferred to a glass slide and stained with
hematoxylin and eosin stains. The slides were then viewed under light microscope
at ×100 and ×400 magnification and photomicrographs were taken at
both magnifications.
Statistical Analysis
Results obtained from the analysis of andrological parameters (Sperm count, sperm
morphology, sperm motility and testosterone concentration), of Sprague-Dawley
rats were statistically analyzed, to see the correlation between the results we
used the Graphpad prism version 5.01. The results were presented as Mean
± SEM (Standard Error of Mean) with significant level at
p-value < 0.05, while the histological examination,
sperm analysis and serum testosterone level were carefully studied and analyzed
to establish any correlation between the groups.
RESULTS
Andrological parameters
The results depicted on Figure 1 indicate
the mean value outcomes of the sperm count, where we found no significant
difference in the mean value of sperm count in Groups B, C, C1 and D1 when
compared with the Control Group A, but with a slight significant increase
(p < 0.05) in Group B1, and this may be due to an
anti-oxidative effect of D-ribose L-cysteine on the low dose Aluminum
administered to Group B rats' testes. Moreover, there was a highly significant
decrease (p < 0.001) in the sperm count value in Group D
rats' given a high dose of Aluminum chloride.
Figure 1
Comparison between the Control and treated groups in terms of sperm
counts after administration of Aluminum chloride and D-ribose
L-cysteine. Group D, showed a highly significant decrease in sperm
count (***p < 0.001); however, Group B1 showed a
slightly significant increase in sperm counts (*p
< 0.05) when compared with the control Group A rats.
Comparison between the Control and treated groups in terms of sperm
counts after administration of Aluminum chloride and D-riboseL-cysteine. Group D, showed a highly significant decrease in sperm
count (***p < 0.001); however, Group B1 showed a
slightly significant increase in sperm counts (*p
< 0.05) when compared with the control Group A rats.The result from Figure 2 shows the sperm
morphology mean value and it was seen that there was no significant difference
in the mean value of sperm morphology (Normal and Abnormal) in Groups B and C1
when compared with the control group A. Moreover, Group B1 rats have slightly
significant increase (p < 0.05) in the numbers of normal
sperm morphology. Group C rats showed slightly significant decreases
(p < 0.05) in the mean values of normal sperm morphology
when compared with the Control Group A, but with the counter administration of
D-ribose L-cysteine (Group C1) the number of normal sperm significantly
increased. Furthermore, Group D rats showed highly significant decreases
(p < 0.001) in the mean value of normal sperm morphology
when compared with the Control Group A, but with the counter administration of
D-ribose L-cysteine (Group D1) the number of normal sperm morphology slightly
increased but not up to the mean value of the Control Group A
(p < 0.01).
Figure 2
There was no significant difference in the mean value of sperm
morphology (Normal and Abnormal) in Group B rats and Group C1 rats,
but a slightly significant increase and decrease in Group B1 and C
rats, respectively. However, a highly significant decrease was
observed in Group D & D1 rats, when compared with the Control
Group A rats (*p < 0.05, **p
< 0.01, ***p < 0.001).
There was no significant difference in the mean value of sperm
morphology (Normal and Abnormal) in Group B rats and Group C1 rats,
but a slightly significant increase and decrease in Group B1 and C
rats, respectively. However, a highly significant decrease was
observed in Group D & D1 rats, when compared with the Control
Group A rats (*p < 0.05, **p
< 0.01, ***p < 0.001).Moreover, Sperm motility mean values from figure
3 shows no significant difference in the mean value of Groups B and
C1 when compared with the control group A. Moreover, Group B1 rats have slightly
significant increases (p < 0.05) in the numbers of motile
sperm. Group C rats showed slightly significant decreases (p
< 0.05) in the mean value of motile sperm when compared with the Control
Group A, but with the counter administration of D-ribose L-cysteine (Group C1)
the number of motile sperm significantly increased. Furthermore, Group D rats
showed highly significant decreases (p < 0.001) in the mean
value of motile sperm when compared with the Control Group A; but with the
counter administration of D-ribose L-cysteine (Group D1) the number of normal
sperm morphology slightly increased, but not up to the mean value of the Control
Group A (p < 0.01).
Figure 3
There was no significant difference in the mean value of sperm
motility in Group B & C rats, but a slight significant increase
and decrease in Group B1 and C rats, respectively. However, a highly
significant decrease was found in Group D & D1 rats when
compared with the Control Group A rats (*p <
0.05, **p < 0.01, ***p <
0.001).
There was no significant difference in the mean value of sperm
motility in Group B & C rats, but a slight significant increase
and decrease in Group B1 and C rats, respectively. However, a highly
significant decrease was found in Group D & D1 rats when
compared with the Control Group A rats (*p <
0.05, **p < 0.01, ***p <
0.001).Furthermore, serum testosterone levels, as shown in figure 4, revealed that there was no significant difference in the
mean value of serum testosterone in Group B rats when compared with the control
group A. Moreover, Group B1 rats showed highly significant increases
(p < 0.001) in the mean value of serum testosterone.
Group C rats showed slightly significant decreases (p <
0.05) in the mean value of serum testosterone when compared with the Control
Group A, but with the counter administration of D-ribose L-cysteine (Group C1)
the mean value of serum testosterone significantly increased (p
< 0.05). Furthermore, Group D rats showed highly significant decreases
(p < 0.001) in the mean value of serum testosterone when
compared with the Control Group A, but with the counter administration of
D-ribose L-cysteine (Group D1) the mean value of serum testosterone still
significantly decreased (p < 0.001) when compare with the
Control Group A.
Figure 4
There was no significant difference in the mean value of Serum
testosterone level in Group B rats, but a slight significant
decrease and increase in Group C & C1 rats, respectively.
However, there was a highly significant increase in Group B1 rats,
while a highly significant decrease was seen in Group D & D1
rats, when compared with the Control Group A rats
(*p < 0.05, *** p <
0.001).
There was no significant difference in the mean value of Serum
testosterone level in Group B rats, but a slight significant
decrease and increase in Group C & C1 rats, respectively.
However, there was a highly significant increase in Group B1 rats,
while a highly significant decrease was seen in Group D & D1
rats, when compared with the Control Group A rats
(*p < 0.05, *** p <
0.001).
Histological Examination of the Testes
Figures 5 and 6 show the histoarchitecture of the testes "stain with H&E" at
x100 and x400 magnification respectively. We found from the slides, that the
Group A, B and C rats' testes appeared normal while severe testicular damages
with several abnormal seminiferous tubules, incomplete maturation of germinal
cell layers(GC), absence of spermatozoa in the lumen (L) and Leydig cells (LC)
hyperplasia were seen in Group D rats. Furthermore, Groups B1, C1 and D1
histological parameters appeared normal.
Figure 5
Histoarchitecture of the testes “stained with H&E”. Group A, B
and C rats appeared normal, while Group D rats showed testicular
damages with several abnormal seminiferous tubules with incomplete
maturation of germinal cell layers(GC) and absence of spermatozoa in
their lumen (L), leydig cells (LC) appeared hyperplastic. Group B1,
C1 and D1 histological parameters appeared normal.
Figure 6
Histoarchitecture of the testes “stained with H&E”. Group A, B
and C rats appeared normal, while Group D rats showed testicular
damages with several abnormal seminiferous tubules with incomplete
maturation of germinal cell layers(GC) and absence of spermatozoa in
their lumen (L), leydig cells (LC) appeared hyperplastic. Group B1,
C1 and D1 histological parameters appeared normal.
Histoarchitecture of the testes “stained with H&E”. Group A, B
and C rats appeared normal, while Group D rats showed testicular
damages with several abnormal seminiferous tubules with incomplete
maturation of germinal cell layers(GC) and absence of spermatozoa in
their lumen (L), leydig cells (LC) appeared hyperplastic. Group B1,
C1 and D1 histological parameters appeared normal.Histoarchitecture of the testes “stained with H&E”. Group A, B
and C rats appeared normal, while Group D rats showed testicular
damages with several abnormal seminiferous tubules with incomplete
maturation of germinal cell layers(GC) and absence of spermatozoa in
their lumen (L), leydig cells (LC) appeared hyperplastic. Group B1,
C1 and D1 histological parameters appeared normal.
DISCUSSION
Aluminum chloride at doses of 75 mg/kg and 150 mg/kg of body weight proved normal in
all the andrological parameters (sperm count, sperm motility, sperm morphology and
serum testosterone), and the testicular histoarchitecture was normal.AlCl3 at a dose of 300 mg/kg body weight was revealed to cause decrease in
the andrological parameters, while some abnormalities were observed in the
histoarchitecture of the testes. This finding is in line with the study of
[Pizent ], in which they reported that aluminum metal affect
spermatogenesis in rodents and humans - which can lead to low sperm count, abnormal
sperm morphology and poor semen quality. Moreover, [Berihu ] revealed that
the reproductive toxicity induced by aluminum is a result of increased in oxidative
stress.D-ribose and L-cysteine (Riboceine) at a dose of 30 mg/kg for all the groups was
found to boost fertility in male Sprague-Dawley rats. D-ribose and L-cysteine at a
dose of 30 mg/kg of body weight significantly boosted andrological parameters in
group B1 and C1 rats treated with 75mg/kg and 150mg/kg of body weight of Aluminum
chloride respectively. Furthermore, D-ribose and L-cysteine at a dose of 30 mg/kg of
body weight moderately boosted reproductive parameters damaged by high dose (300
mg/kg body weight) of Aluminum chloride. The increase in andrological parameters
seen in the B1, C1 and D1 groups after counter treatment with 30 mg/kg of body
weight of D-ribose and L-cysteine may be due to the anti-oxidative protective
effects of D-ribose and L-cysteine. The presence of cysteine in the body's cells
enables the production of glutathione, while ribose produces cellular energy. It is
the interaction between D-ribose and L-cysteine that facilitates the production of
glutathione. The Glutathione within the cell protects against destruction from
free-radical damage. Providing support to Glutathione, improves ATP production by
allowing mitochondria to manufacture ATP, controlling free radicals on an ongoing
basis.
Recommendation
It is therefore recommended that further studies should be carried out to
evaluate molecular mechanisms on which D-Ribose and L-Cysteine (Riboceine) work.
Moreover, D-Ribose and L-Cysteine (Riboceine) is recommended for any infertility
related problems, since it has been revealed from this present study to be a
better antioxidant drug because of its beneficiary effects on males. In
conclusion, D-Ribose and L-Cysteine (Riboceine) have been shown in this present
study to ameliorate the toxic effect of aluminum chloride on the testes, and it
will be a good drug for boosting male fertility because of it potent antioxidant
property.
ADDITIONAL INFORMATION
All the experimental procedures were done following the experimental guidelines of
the Health Research and Ethics Committee (HREC) of the Osun State University, Osogbo
Campus, Osogbo, Osun State.There was no fund or grant received during this research work.This manuscript has been read and approved by all participating authors, thus no
conflict of interests existed.
Authors: Abraham A A Osinubi; Leke Jacob Medubi; Edidiong N Akang; Lawal K Sodiq; Titilola A Samuel; Taiwo Kusemiju; James Osolu; Danladi Madu; Olufemi Fasanmade Journal: Toxicol Rep Date: 2018-08-09
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