Mazdak Razi1, Rajab-Ali Sadrkhanloo1, Hassan Malekinejad2, Farshid Sarafzadeh-Rezaei3. 1. Department of Comparative Histology and Embryology, University of Urmia, Urmia, Iran. 2. Department of Pharmacology and Toxicology, Faculty of Veterinary Medicine, University of Urmia, Urmia, Iran. 3. Department of Clinical Science, Division of Surgery, University of Urmia, Urmia, Iran.
Abstract
BACKGROUND: We designed this study to clarify how varicocele can time-dependently affect sperm morphological parameters and DNA integrity. In this study, we intend to estimate the effect of various periods of varicocele on the in vitro fertilization (IVF) rate in rats. MATERIALS AND METHODS: In this experimental study, left varicocele were induced as the test group (n=18) which was further sub-divided into three groups based on the study termination time (4, 6 and 8 months after varicocele induction). The control-sham group (n=6) consisted of rats who received no treatment. Repopulation index (RI), tubular differentiation index (TDI), sperm viability and motility, morphological maturity, chromatin integrity and ability to undergo IVF were assessed. In addition, the potential impact of varicocele on serum total antioxidant capacity (TAOC) and total thiol molecules (TTM) were examined. RESULTS: Histological results showed that varicocele negatively influenced TDI and RI. All sperm morphological parameters were lower than those in the control-sham group. DNA damage was severely and time-dependently substantiated in all test groups. Varicocele significantly reduced the ability of sperm derived from varicocele rats to undergo IVF. Serum TAOC and TTM levels reduced in a time-dependent manner. Right testes varicocele-induced rats showed remarkably less damaged profile for all investigated parameters compared to the left testes varicocele. CONCLUSION: Our data suggested that experimentally induced varicocele negatively impacted sperm maturation and chromatin integrity in a time-dependent manner. This consequently caused a remarkable reduction in IVF ability. The detrimental effect of varicocele may be attributed to the significant reduction of antioxidant capacity of the serum.
BACKGROUND: We designed this study to clarify how varicocele can time-dependently affect sperm morphological parameters and DNA integrity. In this study, we intend to estimate the effect of various periods of varicocele on the in vitro fertilization (IVF) rate in rats. MATERIALS AND METHODS: In this experimental study, left varicocele were induced as the test group (n=18) which was further sub-divided into three groups based on the study termination time (4, 6 and 8 months after varicocele induction). The control-sham group (n=6) consisted of rats who received no treatment. Repopulation index (RI), tubular differentiation index (TDI), sperm viability and motility, morphological maturity, chromatin integrity and ability to undergo IVF were assessed. In addition, the potential impact of varicocele on serum total antioxidant capacity (TAOC) and total thiol molecules (TTM) were examined. RESULTS: Histological results showed that varicocele negatively influenced TDI and RI. All sperm morphological parameters were lower than those in the control-sham group. DNA damage was severely and time-dependently substantiated in all test groups. Varicocele significantly reduced the ability of sperm derived from varicocele rats to undergo IVF. Serum TAOC and TTM levels reduced in a time-dependent manner. Right testes varicocele-induced rats showed remarkably less damaged profile for all investigated parameters compared to the left testes varicocele. CONCLUSION: Our data suggested that experimentally induced varicocele negatively impacted sperm maturation and chromatin integrity in a time-dependent manner. This consequently caused a remarkable reduction in IVF ability. The detrimental effect of varicocele may be attributed to the significant reduction of antioxidant capacity of the serum.
Entities:
Keywords:
DNA Damage; In vitro Fertilization; Oxidative Stress; Varicocele
Varicocele is defined by abnormal tortuosity and
pampiniform plexus venous dilation within the
spermatic cord and is the most common surgically
correctible cause of male infertility (1, 2). According
to several clinical reports, varicocele is observed
in 10-20 % of the general male population,
35-40% of men with primary infertility and up to
80% of men with secondary infertility (3, 4). Varicoceles
are progressive, often appearing at puberty
and more commonly (90%) located on the left side
(5). Despite numerous studies that have focused
on varicocele, the exact mechanism(s) by which
varicocele induces testicular degeneration, dysfunction
and finally infertility have not completely
understood. The suggested mechanisms include
reflux of toxic metabolites from the adrenal and/
or renal origin, impairment of the hypothalamicgonadal
axis, venous stasis leading to testicular
hypoxia and temperature elevation in the testicles
(6, 7). However, it has long been recognized that
left-sided varicoceles can have bilateral effects (2,
8). The pathophysiologic influence of varicocele
differs depending on the time and exact mechanism
by which this deficiency affects semen parameters. Often, varicocele results in a generalized
degeneration of sperm production (9, 10).A relationship between infertility and the generation
of reactive oxygen species (ROS) has recently
been established and widely studied (11-13). According
to previous reports following different
toxicological, iatrogenic and genetically-induced
degenerations, the mitochondria and plasma membrane
of morphologically abnormal spermatozoa
produce ROS through the nicotinamide adenine dinucleotide
phosphate-dependent and nicotinamide
adenine dinucleotide-dependent oxidoreductase
systems (6, 14).In addition, oxidative stress has been shown to
affect the integrity of the sperm’s genome by causing
high frequencies of single- and double-strand
DNA breaks, often detected in the ejaculates of infertile
men (15-17). Thus, the primary aim of the
present study was to evaluate the concomitant effect
of both left and right testicular varicocele on
spermatogenesis. Secondly, we aimed to estimate
semen quality, sperm DNA fragmentation and the
in vitro fertilizing ability of sperm at various times
following varicocele induction. We also sought to
analyze serum total antioxidant capacity (TAOC)
and total thiol molecules (TTM) in order to clarify
any pathological alterations in serum antioxidant
capacity as well as to illustrate the relationships
of these factors with testicular degeneration and
semen quality during different intervals post-varicocele
induction. In the present study, rats were
selected as a laboratory model for humans.
Materials and Methods
Animals
In this experimental study,twenty-four mature
male Wistar rats, 10 weeks old that weighed 200
± 14 g were used. The rats were purchased from
the Animal Resources Center, Faculty of Veterinary
Medicine, Urmia University, Urmia, Iran
and were acclimatized in an environmentally
controlled room (temperature: 20-23°C and a 12
hours light/12hours dark schedule). Food and
water were available ad libitum. In this study, all
experiments conducted on the animals were in accordance
with Urmia University’s guidance from
the Ethical Committee for Research on Laboratory
Animals. Following one week acclimation,
the animals were assigned to four groups (n=6)
of control-sham and test groups. The test group
was further divided into 3 subgroups according
to the study termination (4, 6 and 8 months) after
varicocele induction.
Varicocele induction
In the test groups, the left varicocele was induced
as previously reported (18). Briefly, following anesthesia
with 5% ketamine (40 mg/kg, i.p.) and
2% xylazine (5 mg/kg, i.p.), the diameter of renal
vein was reduced to 1 mm and a left renal vein
ligation was performed medial to the junction of
the adrenal and spermatic veins. Then, the anastomotic
branches between the left testicular and left
common iliac vein were ligated. The control-sham
group, while under anesthesia, only underwent a
simple laparatomy with no ligation.
Histological analyses
Animals were euthanized on 4, 6 or 8 months following
varicocele induction, by a special CO2 device.
The testes were dissected out, fixed in 10%
formalin fixative for histological investigations and
subsequently embedded in paraffin. Sections (5-6
μm) were stained with Iron-Weigert (Pajohesh Asia,
Iran) for detection of germinal cell nuclei in the testis.
The sections were analyzed under light microscope
at two magnifications (×400 and ×1000).
Tubular differentiation index
To estimate tubular differentiation index (TDI),
the percentage of seminiferous tubules (STs) that
contained more than three layers of differentiated
germinal cells from spermatigonia type A were
considered negative. Those which showed more
than three and/or four layers were considered TDI
positive. From each sample, 20 sections (6 μm)
were prepared and analyzed.
Repopulation index
We used the repopulation index (RI) to calculate
the ratio of active spermatogonia (spermatogonia
type B) with light nuclei to inactive spermatogonia
(spermatogonia type A) with dark nuclei as seen
by Iron-Weigert staining in STs from 20 prepared
sections per sample, as described earlier (19, 20).
Epididymal sperm count, viability, nucleus maturity
and quantitative sperm motility
Epididymides were carefully separated from the
testicles under x20 magnification with a stereo
zoom microscope (Model TL2, Olympus Co.,
Tokyo, Japan). The epididymis was divided into
3 segments: head, body and tail. The epididymal
tail was trimmed and minced in 5 mL Hams F10
medium. After 20 minutes, the ground epididymal
tissue was separated from the released spermatozoa
and counted. Smears were prepared by eosinnegrosin to evaluate dead, abnormal and morphologically
immature sperm (MIS). Sperm which
stained red were considered non-viable; those with
cytoplasmic residuals were considered morphologically
immature.Aniline blue staining was performed in order to
evaluate sperm nuclear maturity (or protamine deficiency).
The proportion of motile spermatozoa
was determined by counting 100 cells in randomly
selected fields for each sample at 37°C (21).
Epididymal sperm DNA fragmentation and double-
strand DNA breaks
The comet assay (Cat No. 1435723/34, Sigma
Co., St. Louis, MO, USA) was used to investigate
DNA fragmentation A ×40 objective device (Olympus,
Germany) was linked to an epi-fluorescent
microscope (Model GS7, Nikon Co., Japan) and
used for visualization of DNA damage. Light green
spots with typical tails were considered to be damaged
DNA and spots with no tails were marked as
normal DNA.To evaluate DNA double strand breaks, an acridine
orange staining kit (Sigma Co., St. Louis, MO,
USA) was used. Samples were analyzed by epifluorescent
microscope (Model GS7, Nikon Co.,
Japan). Sperm samples for acridine orange staining
were provided as previously described (22).
Sperm processing for in vitro fertilization
Samples that contained spermatozoa were prepared
from the sperm suspensions as mentioned
earlier. The samples were incubated at 37°C under
5% CO2 (CO2 Incubator, LEEC, England) for 3
hours. Then, as previously described, 0.1 ml from
superficial sperm and/or 0.1 ml from sediment
sperm of suspensions in one tube were added to
150 μl of tissue culture medium (TCM) that contained
the oocytes (23).
Collection of oocytes and insemination
Mature female rats were injected subcutaneously
with 7.5 IU pregnant mare’s serum hMG (hMG,
Netherlands) 48 hours prior to an i.p. injection
of 100 IU human chorionic gonadotropin hCG
(Teikoku Zohki Co., korea). Rats were euthanized
with a special CO2 device 24 hours after hCG injection.
The oviducts were removed and the ampullar
portion was placed into a plastic dish that
contained PBS (pH=7.2). The oocytes that were in
cumulus masses were dissected out of the oviducts
and introduced into tissue culture medium 199
(TCM 199, Sigma Co., USA). A drop of medium
with 2 oocytes was allocated with a 10 μl sperm
suspension (total: 80,000 sperm). For each animal,
a total of 20 oocytes were divided into 10 drops.
Assessment of serum total antioxidant capacity
To determine the effect of varicocele on oxidative
stress, total antioxidant capacity (TAOC) of
the control-sham and test groups were measured.
The assessment was performed based on the ferric
reduction antioxidant power (FRAP) assay
(19). Briefly, at low pH (acetate buffer, 300 mM,
pH 3.6), reduction of the FeIII-TPTZ complex to
the ferrous form produces an intensive blue color
measurable at 593 nm. The intensity of the complex
following addition of the appropriate volume
of serum to the reducible solution of FeIII-TPTZ is
directly related to the total reducing power of the
electron donating antioxidant. An aqueous solution
of FeII (FeSO4.7H2O) and appropriate concentration
of freshly prepared ascorbic acid are used as
blank and standard solutions, respectively.
Measurement of serum total thiol molecules
The total sulfhydryl level in serum was measured
according to Hu and Dillared method (19). In
short, 0.2 ml serum was added to 0.6 ml Tris-EDTA
buffer (Tris base 0.25 M, EDTA 20 mM, pH=
8.2) followed by the addition of 40 μl DTNB (10
mM in pure methanol) in a 10 ml glass test tube.
The final volume of the mentioned mixture was
made up to 4.0 ml by extra addition of methanol.
After incubation for 15 minutes at room temperature,
the samples were centrifuged at 3000 x g for
10 minutes and ultimately the absorbance of the
supernatant was assessed at 412 nm.
Statistical analyses
Statistical analyses were performed on all numerical
data by two-way ANOVA and SPSS software
version 13.00. All values were expressed as
mean ± SD. P<0.05 was considered statistically
significant.
Results
Light microscopic analyses of the seminiferous
tubules (STs showed most tubules with germinal
epithelium dissociation and disruption of the cellular
junction between sertoli and spermatogenesis
cells. More than 33.50 ± 5.80% of STs in the left
testes and 21.25 ± 2.21% in the right testes .showed
dissociated epithelium after 4 months of varicocele
induction. This phenomenon increased over time; after 6 months, 41.50 ± 3.10% of STs, and at
8 months, 52.25 ± 1.70%, of STs demonstrated cellular
dissociation in the left testes. The right testes
of the test groups showed 34.25 ± 3.09% and 38.12
± 1.93% dissociation in the germinal epithelium of
tubules at 6 and 8 months after varicocele initiation,
respectively. No histological alterations were
noted in the control-sham group and the STs manifested
with normal cellular junction (Fig 1).
Fig 1
Photomicrograph of rat testis. A. Control-sham group.
The seminiferous tubules with normal cellular junction (S)
and interstitial connective tissue without any edema are seen
(I). B. Left varicocelized testis. The dissociated germinal epithelium
in seminiferous tubules (S) with edema in the interstitial
connective tissue is observed (I). Iron-Weigert staining,
(A × 100 and B × 400).
Photomicrograph of rat testis. A. Control-sham group.
The seminiferous tubules with normal cellular junction (S)
and interstitial connective tissue without any edema are seen
(I). B. Left varicocelized testis. The dissociated germinal epithelium
in seminiferous tubules (S) with edema in the interstitial
connective tissue is observed (I). Iron-Weigert staining,
(A × 100 and B × 400).Histological observations demonstrated that most
STs had negative TDI, which further deteriorated with
time in the test groups. The majority of STs showed
depletion and reduction of germinal cell layers after 8
months. Right testes of the test animals showed relatively
moderate destruction in STs when compared to
the left testes. No histological abnormality was observed
in the control-sham group (Fig 2).
Fig 2
Photomicrograph of rat testis. A. Control-sham
group. Note the seminiferous tubules with normal cellular
junction (S) and the interstitial connective tissue with
no edema (I). B. Right testes of varicocelized rats. Note
the seminiferous tubules with negative tubular differentiation
index (S). The spermatogenesis regions (arrowheads)
are indicative of early maturation from the previous cycle.
C. Left testis of varicocelized group. The seminiferous tubules
(S) are completely depleted with no detectable spermatic
maturation. Vascular thrombosis (T) is also observed
in interstitial connective tissue. Iron-Weigert staining, (A ×
100; B × 400 and C × 400).
Special nucleus staining (Iron-Weigert) was performed
in order to differentiate inactive cells (spermatogonia
type A) from active cells (spermatogonia type
B). The results showed that after varicocele induction
the RI was negative in most test group STs and the
number of STs with negative RI increased over time
in both the right and left testes. Although pathologic
RI was present in both testes, the right testes of the
test animals showed lower negative RI in comparison
to the left (Fig 3-A and 3-B). Further analyses showed
some STs with maturation arrest (MA) in the test
groups that were substantiated by time. The quantitative
data for TDI and MA are shown in table 1.
Fig 3
Effect of varicocele on repopulation index in: (A) Left
testis and (B) right testis. Repopulation index percentage of
spermatogonia type A reduced over time in all varicoceleinduced
rats and the spermatogonia type B increased by the
time. Ø and stars indicate significant differences (p ≤ 0.05)
between data for spermatogonia types A and B, respectively.
All data are presented as mean ± SD.
Photomicrograph of rat testis. A. Control-sham
group. Note the seminiferous tubules with normal cellular
junction (S) and the interstitial connective tissue with
no edema (I). B. Right testes of varicocelized rats. Note
the seminiferous tubules with negative tubular differentiation
index (S). The spermatogenesis regions (arrowheads)
are indicative of early maturation from the previous cycle.
C. Left testis of varicocelized group. The seminiferous tubules
(S) are completely depleted with no detectable spermatic
maturation. Vascular thrombosis (T) is also observed
in interstitial connective tissue. Iron-Weigert staining, (A ×
100; B × 400 and C × 400).Effect of varicocele on mean average of tubular differentiation
index and maturation arrest percentage in the
right and left testes of test and control-sham groupsStars indicate significant differences (p≤0.05) between the
control-sham and test groups in the same column. Letters
in the same rows represent significant differences (p≤0.05)
between the left and right testes in same months. All data are
presented as mean ± SD.
Sperm count and morphology
Hemocytometric evaluations for sperm count
showed that after varicocele induction the sperm
number reduced significantly (p<0.05); this reduction
increased with time. Eight month varicoceleinduced
cases manifested severely decreased sperm
count; one of the six rats in this group was azoospermic.
The right testes of varicocele-induced animals
showed relatively higher sperm counts in all test
groups when compared to the left testes. Aniline
blue staining for sperm nucleus maturity revealed
that the ratio of immature sperm with light stained
nuclei increased remarkably in varicocele-induced
animals (Fig 4A). The rats that suffered from varicocele
for 8 months manifested higher numbers or
percentages of immature sperm when compared
with the other test groups. Furthermore, the sperm
with cytoplasmic droplets were considered MIS.
Observations demonstrated that the number of
sperm with cytoplasmic droplets increased significantly
(p<0.05) in varicocele-induced groups. Accordingly,
8 month varicocele-induced rats had the
highest MIS value. In comparison to the left testes,
the right testes showed a lower rate of immature
sperm. A comparison of the results between sperm
collected from the right testes of the varicocele-induced
group with the control-sham group revealed
that MIS was significantly (p<0.05) higher in right
testes samples (Fig 4B).
Fig 4
Light microscopic architecture from sperm; A1; Abnormal
sperm with dense blue stained mature nucleus, A2;
Normal sperm with unstained cytoplasm in head section,
B1; Normal sperm with light stained immature nucleus,
and B2; Abnormal sperm; note the sperm in the left side of
the figure with cytoplasmic droplet (arrows) and the dead
sperm with eosin-stained cytoplasm (below, right hand side).
Aniline-blue (A-1, B-1) and eosin-negrosin (A-2, B-2) stainings,
(× 400).
Light microscopic analyses for sperm motility
showed that the percentage motility decreased
over time in varicocele-induced rats. Sperm delivered
from the right testes of varicocelized animals
exhibited relatively higher sperm motility in comparison
to the left testes.According to the results from eosin-negrosin
staining, there was lower sperm viability in varicocele-
induced rats, with the highest sperm mortality
seen in the 8 month varicocelized animals.
The percentage of viable sperm was also higher
in the right varicocele group when compared with
the left varicocele group. Data for sperm count
and morphology are presented in table 2.Effect of varicocele on: mean average for sperm count (S/C), sperm normality (S/M),
sperm viability (S/V), morphological immature sperm (MIS) and nuclear immature sperm (NIS) in
the different test groups and control-sham groupStars indicate significant differences (p<0.05) between the control-sham and test groups in the same row.Different letters in the same columns are significant differences (p<0. 05) between the right and left testes
in the same month. All data are presented as mean ± SD.Effect of varicocele on repopulation index in: (A) Left
testis and (B) right testis. Repopulation index percentage of
spermatogonia type A reduced over time in all varicoceleinduced
rats and the spermatogonia type B increased by the
time. Ø and stars indicate significant differences (p ≤ 0.05)
between data for spermatogonia types A and B, respectively.
All data are presented as mean ± SD.Effect of varicocele on mean average for DNA
fragmentation and DNA double-strand breaks in the
test groups and control-sham groupStars indicate significant differences (p < 0.05) between the
control-sham and test groups in the same column. Letters
in the same rows indicate significant differences (p ≤ 0.05)
between the left and right testes in the same months. All data
are presented as mean ± SD.Light microscopic architecture from sperm; A1; Abnormal
sperm with dense blue stained mature nucleus, A2;
Normal sperm with unstained cytoplasm in head section,
B1; Normal sperm with light stained immature nucleus,
and B2; Abnormal sperm; note the sperm in the left side of
the figure with cytoplasmic droplet (arrows) and the dead
sperm with eosin-stained cytoplasm (below, right hand side).
Aniline-blue (A-1, B-1) and eosin-negrosin (A-2, B-2) stainings,
(× 400).
Sperm DNA fragmentation and double-strand breaks
Results from the comet assay showed an elevated
ratio of sperm DNA fragmentation in the varicoceleinduced
animals that increased over time. Sperm from
the left varicocelized testes had higher DNA fragmentation
when compared with the right testes in the same
animals and the control-sham group (Fig 5).
Fig 5
Epi-fluorescent architecture of rat sperms by Comet
assay. A. Sperms from control group; the green spots without
any tails are normal sperm. B. Sperms from right testes; The
green spots without tails (arrowhead) and spots with tails
(arrow) indicate the DNA fragmentation. In panel B both
normal and fragmented DNA are seen in sperms collected
from the right testes of varicocelized rats, C. Sperms collected
from the left testes of varicocelized rats with intensive
DNA fragmentation; (Comet assay technique, × 100).
Epi-fluorescent architecture of rat sperms by Comet
assay. A. Sperms from control group; the green spots without
any tails are normal sperm. B. Sperms from right testes; The
green spots without tails (arrowhead) and spots with tails
(arrow) indicate the DNA fragmentation. In panel B both
normal and fragmented DNA are seen in sperms collected
from the right testes of varicocelized rats, C. Sperms collected
from the left testes of varicocelized rats with intensive
DNA fragmentation; (Comet assay technique, × 100).Acridine-orange staining showed that the number
of sperm with double-strand DNA breaks was significantly
(p<0.05) higher in the varicocelized
groups with the highest rate of DNA breaks seen
in rats with 8 months varicocelized testes. The percentage
of DNA breaks was significantly (p<0.05)
lower in sperm from the right testes of varicocelized
animals when compared to samples from the left
testes (Fig 6). The numerical data for sperm DNA
fragmentation and breaks are presented in table 3.
Fig 6
Effect of varicocele on double strand DNA in rat
sperm. A. Epi-fluorescent architecture of the control-sham
group. The light green stained nuclei are indicative of the
normal double-strand DNA in this group. B. Light microscopic
architecture of sperm from right testes of varicoceleinduced
rats. The normal sperm with light green stained
nucleolus (arrows) and sperm with damaged DNA with light
yellow stained nucleolus (arrowheads) are presented. C.
Light microscopic architecture of sperm from left testis of
varicocele-induced rat, the sperm with light yellow stained
nucleolus represent remarkable DNA damage (Acridineorange
staining, × 400).
Effect of varicocele on double strand DNA in rat
sperm. A. Epi-fluorescent architecture of the control-sham
group. The light green stained nuclei are indicative of the
normal double-strand DNA in this group. B. Light microscopic
architecture of sperm from right testes of varicoceleinduced
rats. The normal sperm with light green stained
nucleolus (arrows) and sperm with damaged DNA with light
yellow stained nucleolus (arrowheads) are presented. C.
Light microscopic architecture of sperm from left testis of
varicocele-induced rat, the sperm with light yellow stained
nucleolus represent remarkable DNA damage (Acridineorange
staining, × 400).Effect of varicocele on means average of 4- and 8-cell embryos, moru- la and blastocysts after in vitro insemination of oocytes with superficial and sediment sperm contents of the right and left testes from the test and control- sham groupsStars and # indicate significant differences (p < 0.05) between data in the same column with control-sham rats; different letters indicate significant differences (p < 0.05) between data of superficial sperm and sediment sperm contents. All data are presented as mean ± SD. A total of 20 oocytes were used for each sperm sample and the percentages in the table were calculated from 20 oocytes.
Varicocele influences the rate of in vitro fertilization
The results for in vitro fertilization(IVF) of oocytes
by sperm collected from the right and left testes of
varicocelized animals were remarkably lower than
the control-sham group (Fig 7A, B). The considerable
point was that most of the 2-cell embryos arrested
at the first cleavage stage and did not continue
further in the varicocelized group. This phenomenon
was at its highest rate in samples from the left testes
of the varicocelized animals for 8 months. The
results for sperm collected from the upper side of
the tube (superficial sperm) in terms of progress
in cell division were significantly (p<0.05) higher
than those collected from the lower side of the tube
(sediment sperm). A comparison of the values for
fertilization rates between all test groups indicated
that the highest value belonged to oocytes exposed
to sperm from the right testes of varicocelized animals
for 4 months. Therefore, in varicocelized animals
the rate of the morula and blastocysts phases
compared to the control-sham group declined significantly
(p<0.05). The data for IVF rates are presented
in table 4.
Fig 7
Effect of varicocele on IVF and 2-cell embryo after invitro
fertilization in the control and varicocele-induced rats:
A. Left testicle data, B. right testicle data. Stars indicate significant
differences (p ≤ 0.05) between all data for different
months following varicocele induction with each test group
and the control group. All data are presented as mean ± SD.
Alterations in TAOC and TTM
Results indicated that both TAOC and TTM
significantly (p<0.05) decreased after varicocele
induction for 4, 6 and 8 months compared to the
control-sham group. Accordingly, animals in the 8
month varicocele-induced group showed remarkable
diminished antioxidant capacity of serum
(Fig 8 A, B).
Fig 8
Effect of varicocele on the serum level of TAOC (A)
and TTM (B); Stars indicate significant differences (p ≤
0.05) between control and test groups. All data are presented
as mean ± SD.
Effect of varicocele on IVF and 2-cell embryo after invitro
fertilization in the control and varicocele-induced rats:
A. Left testicle data, B. right testicle data. Stars indicate significant
differences (p ≤ 0.05) between all data for different
months following varicocele induction with each test group
and the control group. All data are presented as mean ± SD.Effect of varicocele on the serum level of TAOC (A)
and TTM (B); Stars indicate significant differences (p ≤
0.05) between control and test groups. All data are presented
as mean ± SD.
Discussion
In the present study we showed that in varicoceleinduced
rats there were early MI, negative TDI and
RI due to disrupted spermatogenesis in both the
left and right testes. The negative impact of varicocele
increased over time. Our further analyses
illustrated that following varicocele-induction, in
addition to a reduction in sperm motility, sperm
protamine-histone transition, DNA and plasma
membrane integrity were impaired with a subsequent
loss of motility that increased over time.
Ultimately, our results showed that the quality of
sperm content reduced with time, which in turn reduced
the IVF rate.Varicocele is a disorder with an incidence of 10%
to 20% in the general population (24) that is commonly
diagnosed among men with infertility (25).
Various factors associated with varicocele may
lead to DNA damage, including: heat stress (26,
27), androgen deprivation (6, 28), exposure to toxic
agents (29, 30), testicular hypoxia (31, 32) and
increased oxidative stress (7, 33). In the present
study, we have used specific methods to clarify
the effect of the duration of varicocele and consequently
the probable effect of varicocele-induced
oxidative stress on sperm morphology, maturation
and DNA integrity. We also sought to identify the
IVF ability of these sperm during different time
periods.According to our findings, varicocele does not
exert its pathologic effect immediately, but rather it
takes time to see the various pathological features
associated with varicocele. In many pathological
conditions, apoptosis of germinal cells in STs is the
main cause of germ cell loss and this impairment
can also influence sertoli cells (34-37). According
to several independent reports, high scrotal temperatures
and/or elevated oxidative stress in spermatogenesis
results in apoptosis, thus leading to
remarkable cellular depletion in STs (38-40). Our
findings are in concordance with these reports. We
have illustrated that after varicocele initiation, the
RI ratio in STs is negative, which indicates severe
degeneration in spermatogonia cells. Furthermore,
our light microscopic analyses have shown an intensive
cellular disruption and substantial STs
depletion in the majority of STs in varicocelized
animals as well as severe damage in sertoli cells.
Interestingly, due to hypospermtogenesis and high
MI occurrence, the total sperm content and percentage
of sperm maturity significantly reduced in
varicocele cases over time.In damaged spermatogenesis, the cytoplasmic
extrusion mechanisms do not function normally
(19). In this condition the released spermatozoa
from the germinal epithelium carry surplus residual
cytoplasm and can be counted as immature and functionally defective spermatozoa (19, 20, 41,
42). It is well documented that the level of ROS
production correlates negatively with sperm quality
in the original semen (43, 44).In the current study, samples obtained from 4
month varicocelized rats contained MIS with cytoplasmic
droplets (residual cytoplasm). The rate
of immature sperm occurrence was found to correlate
with imbalance in oxidative defense of the
8 month varicocelized rats. Therefore, the rate of
immature sperm was higher in the samples with
lowest TTM and TAOP. Evidence has shown that
any disruption in the physiological function of
the cytosolic enzyme glucose-6-phosphate-dehydrogenase,
the enzyme that mediates some physiological
bioactivities involved in sperm maturity,
can influence sperm maturity processes in varicocele
patients (42). Interestingly in this study, after
4 and 6 months serum TAOC and thiol molecules
decreased in comparison to control cases, but this
reduction was not statistically significant (p>0.05).
The intensive and remarkable reduction in TTM
and TAOP levels as biomarkers of oxidative stress
occurred 8 months following varicocele induction.
Sperm immaturity and abnormality may have significantly
increased independently to serum antioxidant
capacity from 4 months following varicocele
induction, which progressed over time. Thus,
these findings may suggest that the pathological effect
observed in early varicocele is independent of
reduced sperm antioxidant capacity while the later
effects of varicocele may be increased due to reduced
serum antioxidant capacity. Thus our results
confirm the fact that in varicocelized animals the
extent of damage caused by ROS on sperm parameters
depends not only on the nature and amount of
ROS involved but also on duration of ROS exposure.
According to earlier studies, increased ROS
formation has been correlated with a reduction of
sperm motility (45-47). The link between ROS and
reduced motility can be explained by two hypotheses.
First, a wave of events that result in an intensive
decrease in axonemal protein phosphorylation
and sperm immobilization, and secondly, free
radicals such as H2O2 which can diffuse across the
membranes into cells and inhibit the activities of
enzymes such as glucose 6-phosphate dehydrogenase
(48, 49). Our observations have demonstrated
that after 8 months the varicocele-induced rats
manifested a high percentage of immotile sperm.
This may have occurred because spermatozoa are
particularly susceptible to ROS stress since their
plasma membranes are enriched with unsaturated
fatty acids, particularly decosohexaenoic acid with
six double bonds per molecule. In order to exactly
identify the rate of sperm plasma membrane damage,
eosin-negrosin staining was performed which
confirmed this hypothesis showing an increased
number of sperm with defective plasma membranes.A number of studies have suggested that the presence
of spermatozoa with damaged DNA may be
the result of impaired chromatin packing or indicative
of apoptosis (50, 51). There are external
factors such as transitional changes in the concentration
of trace elements that promote oxidative
stress impact and DNA damage. The protamination
status of chromatin can remarkably protect
sperm from these damages (52, 53). Protamines
may act as protective elements by sequestering
trace elements capable of promoting the fragmentation
of sperm DNA (54). Our special staining for
protamine showed that after varicocele induction,
the protamine-histone transition was impaired
which may have partially accounted for the extensive
DNA damage observed in poorly packaged
spermatozoa of the varicocelized rats. On the other
hand, results from the comet assay and acridine
orange stainings were in accordance with these
findings and showed an elevated sperm DNA fragmentation
and damage in varicocele-induced rats.Reports have indicated that disorders which have
resulted in failure of epididymal sperm maturation
also impair sperm fertilizing ability (40, 48,
50, 55). It is well known that during the epididymal
transition sperm acquires it ability to present
forward motility, undergo capacitation and finally
penetrate the zona pellucida (21). Our observations
have revealed that during long time varicocele,
MIS increased remarkably.According to our results the unsaturated fatty acids
in plasma membrane of sperms were severely
damaged after varicocele induction. These unsaturated
fatty acids are essential for fluidity for the
plasma membrane in order to participate in membrane
fusion events associated with fertilization.
When the associated double bonds with unsaturated
fatty acids deform, the membrane fluidity decreases
and it leads to a consequent loss of sperm
function. Of note, the lowest results for IVF were
manifested after 8 months.The ability of the embryo to survive appears to
be negatively correlated with the level of DNA
fragmentation in the germ line (56). Previous
studies have shown that DNA-damaged sperm can
not fertilize an oocyte (54, 57). Our results in this
study have shown that by using sperm from varicocelized
rats some of the fertilized eggs stopped at the 2-cell embryo phase. The ultimate outcome of
IVF in comparison to the control group was found
remarkably low.
Conclusion
Our data suggest that following varicocele induction
severe damage occurs in the process of spermatogenesis
which influence produced spermatozoa
quality, maturation (testicular and epididimal)
and DNA integrity. On the other hand, increasing
impaired and abnormal sperm leads to remarkable
ROS stress that can result in sperm plasma membrane
disintegrity. Ultimately these impairments
affect sperm capacitation. It may be concluded that
for IVF purposes either sperm samples from varicocele
patients should not be used or sperm samples
that are collected early could be used after testing
for DNA integrity.
Table 1
Effect of varicocele on mean average of tubular differentiation
index and maturation arrest percentage in the
right and left testes of test and control-sham groups
Tubular differentiation index (TDI, %)
Groups
Left testicle
Right testicle
Control-sham
2.25 ± 1.00
2.75 ± 0.95
4 months
23.25 ± 3.59*b'
14.5 ± 3.31*a'
6 months
33.5 ± 3.41*b
23.25 ± 3.59*b'
8 months
37.87 ± 2.65*c
32.50 ± 3.10*c'
Maturation arrest (MA%)
Control-sham
0.7±0.44
0.75 ± 0.28
4 months
33.6±3.57*a
25.50 ± 1.91*a'
6 months
39.2±1.92*
38.5 ± 1.29*
8 months
44.6±3.20*b
40.25 ± 1.70*b'
Stars indicate significant differences (p≤0.05) between the
control-sham and test groups in the same column. Letters
in the same rows represent significant differences (p≤0.05)
between the left and right testes in same months. All data are
presented as mean ± SD.
Table 2
Effect of varicocele on: mean average for sperm count (S/C), sperm normality (S/M),
sperm viability (S/V), morphological immature sperm (MIS) and nuclear immature sperm (NIS) in
the different test groups and control-sham group
Left testes
Parameters
Control-sham
4 months
6 months
8 months
S/C (×106)
72.50 ± 3.78
42.50 ± 2.08*a
38.00 ± 2.16*b
31.75 ± 2.36*c
S/M-%
92.25 ± 1.70
91.00 ± 1.41*a
39.75 ± 1.70*b
33.75 ± 2.62*c
S/V- %
92.33 ± 2.08
57.34 ± 5.03*a
44.66 ± 4.16*b
32.34 ± 2.51*c
MIS-%
16.20 ± 4.43
50.80 ± 1.64*a
59.20 ± 1.66*b
70.20 ± 1.78*c
NIS-%
9.25 ± 0.95
48.75 ± 2.21*a
57.00 ± 1.82*b
62.25 ± 1.70*c
Right testes
S/C(×106)
73.75 ± 3.30
54.50 ± 3.41*a'
43.75 ± 2.06*b'
37.25 ± 1.70*c'
S/M-%
91.25 ± 1.50
56.75 ± 1.70*a'
44.00 ± 3.65*b'
36.00 ± 4.08*c'
S/V-%
92.60 ± 3.05
70.66 ± 3.05*a'
61.34 ± 3.05*b'
44.67 ± 4.16*c'
MIS-%
15.80 ± 5.63
48.60 ± 1.67*a'
55.60 ± 2.60*b'
62.80 ± 2.77*c'
NIS-%
9.26 ± 1.70
42.50 ± 2.51*a'
46.25 ± 2.36*b'
53.72 ± 3.30*c'
Stars indicate significant differences (p<0.05) between the control-sham and test groups in the same row.
Different letters in the same columns are significant differences (p<0. 05) between the right and left testes
in the same month. All data are presented as mean ± SD.
Table 3
Effect of varicocele on mean average for DNA
fragmentation and DNA double-strand breaks in the
test groups and control-sham group
DNA fragmentation (comet assay,%)
Groups
Left testes
Right testes
Control-sham
4.20 ±0.83
4.40±1.14
4 months
35.0±2.30*a
30.60±1.14*b
6 months
41.20±1.30*a
37.00±0.70*b
8 months
53.40±3.28*a
48.80±1.30*b
Maturation arrest (MA%)
Control-sham
3.00±0.70
3.20±0.70
4 months
34.60±3.43*a
28.20±1.78*b
6 months
39.80±1.48*a
34.00±3.39*b
8 months
45.80±1.92*a
41.20±1.78*b
Stars indicate significant differences (p < 0.05) between the
control-sham and test groups in the same column. Letters
in the same rows indicate significant differences (p ≤ 0.05)
between the left and right testes in the same months. All data
are presented as mean ± SD.
Table 4
Effect of varicocele on means average of 4- and 8-cell embryos, moru- la and blastocysts after in vitro insemination of oocytes with superficial and sediment sperm contents of the right and left testes from the test and control- sham groups
Groups
4-cell embryo
Left testes8-cell embryo
Morula
Blastocyst
Control-sham
27.80 ± 2.94
24.20 ± 0.83
22.06 ± 1.67
20.50 ± 1.04
4 months
13.66 ± 2.25*a
12.20 ± 1.64*b
11.40 ± 0.84*c
11.20 ± 0.83*d
6 months
5.50 ± 1.16*
5.80 ± 1.30*
5.60 ± 1.07*c
5.40 ± 2.50*d
8 months
4.83 ± 0.75*a
3.40 ± 1.34*b
3.00 ± 0.70*c
2.80 ± 0.83*d
Sediment sperm content from left testes (%)
Control-sham
27.16 ± 1.47
24.40 ± 1.14
22.60 ± 1.14
19.83 ± 0.75
4 months
11.80 ± 1.48*a'
10.60 ± 1.14*b'
9.20 ± 0.83*c'
9.00 ± 1.41*d'
6 months
5.00 ± 1.41*
4.20 ± 1.09*
4.00 ± 0.70*c'
3.80 ± 0.44*d'
8 months
1.40 ± 0.89*a'
1.30 ± 0.83*b'
1.20 ± 1.09*c'
0.60 ± 0.54*d'
Superficial sperm content from right testes (%)
Groups
4-cell embryo
8-cell embryo
Morula
Blastocyst
Control-sham
27.60 ± 1.81
24.80 ± 1.48
20.80 ± 0.83
19.80 ± 1.14
4 months
14.00 ± 1.00#e
12.37 ± 1.52#f
12.00 ± 1.00#g
11.57 ± 0.95#h
6 months
8.33 ± 1.15#e
8.00 ± 1.00#f
7.66 ± 0.57#g
7.00 ± 0.81#h
8 months
6.34 ± 0.57#e
5.25 ± 0.50#f
4.60 ± 0.57#g
4.25 ± 0.95#h
Sediment sperm content from right testes (%)
Control-sham
27.33±1.03
24.83 ± 1.47
21.50 ± 1.04
19.84 ± 1.47
4 months
13.25±1.25#e'
12.10 ± 0.84#f'
10.62 ± 0.47#g'
9.98± 0.14#h'
6 months
7.50±1.29#e'
6.75 ± 0.95#f'
5.70 ± 0.94#g'
5.00 ± 0.08#h'
8 months
4.50±1.29#e'
9.25 ± 0.95#f'
2.20 ± 0.54#g'
2.25 ± 0.51#h'
Stars and # indicate significant differences (p < 0.05) between data in the same column with control-sham rats; different letters indicate significant differences (p < 0.05) between data of superficial sperm and sediment sperm contents. All data are presented as mean ± SD. A total of 20 oocytes were used for each sperm sample and the percentages in the table were calculated from 20 oocytes.
Authors: Fábio F Pasqualotto; Antônio M Lucon; Jorge Hallak; Plínio M Góes; Luiz B Saldanha; Sami Arap Journal: Hum Reprod Date: 2003-01 Impact factor: 6.918
Authors: Felipe Dieamant; Claudia G Petersen; Ana L Mauri; Vanessa Conmar; Mariana Mattila; Laura D Vagnini; Adriana Renzi; Bruna P Costa; Camila Zamara; João Batista A Oliveira; Ricardo L R Baruffi; José G Franco Journal: JBRA Assist Reprod Date: 2017-12-01
Authors: Niloofar Sadeghi; Naeem Erfani-Majd; Marziyeh Tavalaee; Mohammad R Tabandeh; Joël R Drevet; Mohammad H Nasr-Esfahani Journal: Oxid Med Cell Longev Date: 2020-04-13 Impact factor: 6.543
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