Elsayed A Mohamed1,2, Ji Woo Im1, Dong-Hwan Kim3, Hae-Rahn Bae1. 1. Dept. of Physiology, College of Medicine, Dong-A University, Busan 49201, Korea. 2. Dept. of Genetics, Assiut University, Assiut 71526, Egypt. 3. Human Life Research Center, Dong-A University, Busan 49315, Korea.
Aquaporins (AQPs) are a family of critical transmembrane proteins consisting of
thirteen sub-types (AQP0-12) that are found in most living organisms including
humans, animals, plants, and even lower organisms (Verkman, 2012; Shivaraj et al.,
2017; Azad et al., 2021). In
mammals, this protein family is ubiquitously expressed in various tissues and
secretory glands specifically transferring water, glycerol, urea, or other soluble
molecules across the cell membrane in a bidirectional manner to facilitate fluid
absorption and secretion (Arnaoutova et al.,
2008; Delporte, 2017). AQPs are
playing an important role in the regulation of many cellular physiological processes
including cell migration and proliferation (Meli
et al., 2018), body water homeostasis (Yu et al., 2014), exocrine fluid secretion (Verkman, 2012), and transport the nutrients and other
functional molecules into the cell, as well as elimination of metabolic residues
(Ribeiro et al., 2021).Many reports have demonstrated the expression of AQP proteins in the male
reproductive system in different mammalian species such as humans (Pastor-Soler et al., 2001), rodents (Calamita et al., 2001a, 2001b; Lu et al.,
2008; Ford et al., 2014),
Bactrian camel (An & Wang 2016),
stallion (Klein et al., 2013), bat (Oliveira et al., 2013), cat (Arrighi & Aralla 2014), and dog (Domeniconi et al., 2007). The expression and
localization of AQP proteins in the male reproductive tissues are variable among the
tested mammalian species (Boj et al., 2015;
Carrageta et al., 2020; Ribeiro et al., 2022). However, it has been
repeatedly addressed a potential role of AQPs in spermatozoa osmoregulation,
transition, and concentration, as well as sperm maturation via regulating water
homeostasis and fluid transport in the testes and male reproductive ductules (Lu et al., 2008; Alves et al., 2015; Carrageta et al., 2020). In support of this speculations, the deficiency
or alterations in AQPs expression have been reported to be associated with sperm
dysfunction and male sub-fertility. Chen et al.
(2011) reported that AQP3 deficiency resulted in in
utero sperm tail deformation and impairing male fertility in the
AQP3-knockout mice. Also, the expression of AQP5 was found to be downregulated in
the caput epididymidis from men with nonobstructive azoospermia compared to those
from fertile men (Dube et al., 2008).
Additionally, alteration of the AQP7 expression in infertile patients’sperm
was found to be correlated with lower sperm motility, as well as abnormal sperm
morphology and concentration (Saito et al.,
2004; Yeung et al., 2010; Moretti et al., 2012). On the other hand, in
a contradictory study, Sohara et al. (2007)
reported that AQP7 knockout male mice were not sterile, and their sperm did not show
any morphological or functional abnormalities. Moreover, although the knockout
animals for some other AQP isoforms have been established and studied, their
fertility has not been studied yet (Carrageta et
al., 2020). Therefore, the role of these AQPs in sperm function and male
fertility remains to be elucidated.Although many efforts have been made to study the expression of AQPs in the male
reproductive system using different assays, there is still a lack of the detailed
expression location of these AQPs in the target cells along the male reproductive
tissues (Carrageta et al., 2020; Ribeiro et al., 2022). Elucidating the
detailed expression of the AQP proteins in the testes is a preliminary step to
understand the functions of these AQPs in sperm production and maturation, and hence
male fertility. Therefore, in order to extend the knowledge of the detailed
expression and localization of AQPs, we investigated the expression pattern as well
as the localization of different AQP subtypes in the adult mouse testes and
testicular spermatozoa using an immunofluorescence assay.
MATERIALS AND METHODS
Animals
A total of 6 adult males of CD1 mice aged 10–16 weeks were used in the
present study. The mice were kept at the animal resource center of Dong-A
University Medical School with controlled lighting (12 h light/12 h dark) at a
temperature of 20±2°C and humidity of 50±2%. The animals
were provided with laboratory feed (SAM #31; Samtako, Osan, Korea) and water
ad libitum. The protocols for this study were approved by
Dong-A University Medical School Institutional Animal Care Use Committee
(DIACUC-07-20).
Tissue preparation and frozen sections
The mice were euthanized by cervical dislocation. Then, the testes were exposed
by laparotomy and meticulously isolated. After that, the tissue samples were
embedded in Optimal Cutting Temperature medium (OCT) and rapidly frozen with
liquid nitrogen. To prepare the sections, unfixed OCT-embedded frozen tissue
blocks were sectioned at 5 μm thickness using a cryostat (Leica CM1950,
Leica Biosystems, Nussloch, Germany). Hematoxylin and eosin staining following
standard procedures was used for quality verification of the frozen sections.
Then, the sections were mounted using VectaMount mounting medium (Vector
Laboratories, Burlingame, CA, USA), and then observed using microscopy (BX51,
Olympus, Tokyo, Japan). For further evaluation the slides were scanned with
Panoramic MIDI digital slide scanner (3DHistech, Budapest, Hungary) and images
were analyzed using CaseViewer.
Immunofluorescence
The frozen sections were air-dried and fixed with ice-cold acetone for 30 min at
−20°C. Then they were blocked with 1% bovine serum albumin in PBS
containing 0.025% Tween 20 for 4 h at room temperature. The sections were
incubated with the following primary antibodies overnight at 4°C;
anti-AQP1 (1:200, Chemicon, Temecula, CA, USA), anti-AQP3 (1:200, Chemicon),
anti-AQP7 (1:200, Novus Biologicals, Colorado, CO, USA), anti-AQP8 (1:300,
Mybiosource, CA, USA), anti-AQP9 (1:200, Alpha Diagnostic Intl., San Antonio,
TX, USA), and vimentin (1:200, Santa Cruz Biotechnology, Dallas, TX, USA)
antibodies. After that, the sections were incubated with Alexa Fluor 488 or
594-conjugated anti-rabbit IgG H&L secondary antibodies (1:200,
Invitrogen, Carlsbad, CA, USA) for 1 h at room temperature. Finally, the cell
nuclei were counterstained with Hoechst 33342 trihydrochloride (1:500, Molecular
Probes, Alameda, CA, USA). The sections were then mounted with prolong live
antifade reagent (Invitrogen) and visualized using laser scanning confocal
microscope (LSM 800, Carl Zeiss, Oberkochen, Germany).
RESULTS
The expression and localization of different AQP subtypes (AQP1, AQP3, AQP7, AQP8,
and AQP9) in the adult mouse testes were explored using immunofluorescence assay.
All the AQPs studied were expressed in the testes and revealed subtype-specific
patterns in the expression intensity and localization depending on the cell types of
the testes (Fig. 1). The overall expression
intensity was highest in AQP7, followed by descending order of AQP3, AQP8, AQP9, and
AQP1.
Fig. 1.
The overall expression patterns of AQP subtypes in frozen sections of the
mouse testes.
Hematoxylin and eosin (H/E) stain and immunofluorescence staining of AQP1,
AQP3, AQP7, AQP8, and AQP9 in the mouse testes (n=4). AQPs labeled with red
color and cell nuclei counterstained with Hoechst 33342 (blue color). Note
AQP subtype-specific patterns in the expression intensity and localization
depending on the cell types of the testes. All bars represent 100 μm.
AQP, aquaporins.
The expression intensity of AQP1 was the lowest in general among the tested AQPs.
AQP1 was barely expressed in the germinal epithelium of seminiferous tubules, and
weakly expressed in the interstitial Leydig cells. However, clear labeling of AQP1
was detected in the lumen of seminiferous tubules, corresponding to the tail and
pericentriolar region of the testicular spermatozoa (Fig. 2).
Fig. 2.
The expression of AQP subtypes in the mouse germinal epithelium and
interstitial Leydig cells.
Hematoxylin and eosin (H/E) stain and immunofluorescence staining of AQP1,
AQP3, AQP7, AQP8, and AQP9 in the mouse testes (n=4). AQPs labeled with red
color and cell nuclei counterstained with Hoechst 33342 (blue color).
Interstitial, basal and lower adluminal compartments of the seminiferous
tubule (second row); upper adluminal compartment and lumen of the
seminiferous tubule (third row). White and black arrow heads indicate Leydig
cells and spermatogonia, respectively. White and black arrows indicate
spermatocytes and spermatid, respectively. Note AQP subtype-specific
patterns in the expression intensity and localization depending on the cell
types of the testes. The bars represent 50 μm and 10 μm. AQP,
aquaporins.
The expression intensity of AQP3 was relatively high with broad distribution in the
testis. Inside the seminiferous tubules, AQP3 expression was not with the same
intensity. The strong AQP3 intensity was observed in the basal compartment of the
tubules, corresponding to the spermatogonia and primary spermatocytes as well as
Sertoli cells. Almost no signal was observed in the adluminal compartments. AQP3
expression was also observed in the lumen of the tubules, which coincides with tails
of spermatozoa and elongated spermatids. Moreover, the expression of AQP3 was
observed in the interstitial Leydig cells.Intestingly, AQP7 was the most abundant AQP subtype among the tested AQPs that highly
expressed in both intratubular and peritubular compartments of the seminiferous
tubules. AQP7 was expressed in the all stages of germ cells of basal and adluminal
compartments as well as in the Sertoli cells. Moreover, a strong AQP7 expression was
also observed in the spermatids as well as in the head, pericentriolar region, and
tail of the testicular spermatozoa.AQP8 displayed a characteristic expression with localization to the basal compartment
of the seminiferious tubules, corresponding to spermatogonia. AQP8 was also
expressed in the interstitial Leydig cells with weak signals in the lumen.
The overall expression patterns of AQP subtypes in frozen sections of the
mouse testes.
Hematoxylin and eosin (H/E) stain and immunofluorescence staining of AQP1,
AQP3, AQP7, AQP8, and AQP9 in the mouse testes (n=4). AQPs labeled with red
color and cell nuclei counterstained with Hoechst 33342 (blue color). Note
AQP subtype-specific patterns in the expression intensity and localization
depending on the cell types of the testes. All bars represent 100 μm.
AQP, aquaporins.
The expression of AQP subtypes in the mouse germinal epithelium and
interstitial Leydig cells.
Hematoxylin and eosin (H/E) stain and immunofluorescence staining of AQP1,
AQP3, AQP7, AQP8, and AQP9 in the mouse testes (n=4). AQPs labeled with red
color and cell nuclei counterstained with Hoechst 33342 (blue color).
Interstitial, basal and lower adluminal compartments of the seminiferous
tubule (second row); upper adluminal compartment and lumen of the
seminiferous tubule (third row). White and black arrow heads indicate Leydig
cells and spermatogonia, respectively. White and black arrows indicate
spermatocytes and spermatid, respectively. Note AQP subtype-specific
patterns in the expression intensity and localization depending on the cell
types of the testes. The bars represent 50 μm and 10 μm. AQP,
aquaporins.AQP9 expression was also distinctive, which was confined to the lumen of in the
seminiferous tubules. Strong AQP9 expression was exclusively observed in tails of
the testicular spermatozoa and elongated spermatids. Higher magnification revealed
weak AQP9 expression in the Leydig cells.In order to get more information on the detailed localization of AQP3, AQP7, and AQP8
expressions in interstitial and basal compartments of the seminiferous tubules,
colcalization analysis of these AQPs was performed with vimentin, which is the most
commonly used marker for Sertoli cells. AQP3 expression was identified in
undifferentiated spermatogonia, proliferating primary spermatocytes, Sertoli cells
as well as Leydig cells (Fig. 3). AQP7 was also
expressed in the same cell types as AQP3, but the intensity of AQP7 was stronger
than that of AQP3. AQP8 expression was limited to the spermatogonia and Leydig
cells.
Fig. 3.
Double immunofluorescence of different AQP subtypes and vimentin in the
mouse testes.
AQPs labeled with red color, vimentin labeled with green color and cell
nuclei counterstained with Hoechst 33342 (blue color). Expression levels of
AQP3, AQP7, and AQP8 were compared by interstitial, basal and upper luminal
compartments of the seminiferous tubules of mouse testes (n=2). White and
black arrow heads indicate Leydig cells and spermatogonia, respectively
while white arrows indicate spermatocytes. Note that both AQP3 and AQP7 were
expressed in spermatogonia, proliferating primary spermatocytes, Sertoli
cells as well as Leydig cells, whereas AQP8 was expressed only in the
spermatogonia and Leydig cells. The bars represent 100 μm and 10
μm. AQP, aquaporins.
Relative expression levels of AQP subtypes in interstitial, basal and adluminal
compartments of the seminiferous tubules were quantified in Fig. 4. Leydig cells in interstitial compartment expressed AQP7
at the highest level, followed by AQP8 and AQP3. Spermatogonia and primary
spermatocytes in basal compartment expressed both AQP7 and AQP8 most abundantly,
followed by AQP3. Spermatids and spermatozoa in adluminal compartment expressed AQP7
at the highest level, followed by AQP9 and AQP3.
Fig. 4.
Relative expression levels of AQP subtypes in the seminiferous tubules of
the mouse testes.
Confocal immunofluorescence images of AQP1, AQP3, AQP7, AQP8, and AQP9 were
anlayzed by the automated determination of mean fluorescence intensity of
cells expressing AQP subtypes in interstitial, basal and adluminal
compartments of the seminiferous tubules. The data represent mean±SE
of 4 invididual experiments. AQP, aquaporins.
Double immunofluorescence of different AQP subtypes and vimentin in the
mouse testes.
AQPs labeled with red color, vimentin labeled with green color and cell
nuclei counterstained with Hoechst 33342 (blue color). Expression levels of
AQP3, AQP7, and AQP8 were compared by interstitial, basal and upper luminal
compartments of the seminiferous tubules of mouse testes (n=2). White and
black arrow heads indicate Leydig cells and spermatogonia, respectively
while white arrows indicate spermatocytes. Note that both AQP3 and AQP7 were
expressed in spermatogonia, proliferating primary spermatocytes, Sertoli
cells as well as Leydig cells, whereas AQP8 was expressed only in the
spermatogonia and Leydig cells. The bars represent 100 μm and 10
μm. AQP, aquaporins.
Relative expression levels of AQP subtypes in the seminiferous tubules of
the mouse testes.
Confocal immunofluorescence images of AQP1, AQP3, AQP7, AQP8, and AQP9 were
anlayzed by the automated determination of mean fluorescence intensity of
cells expressing AQP subtypes in interstitial, basal and adluminal
compartments of the seminiferous tubules. The data represent mean±SE
of 4 invididual experiments. AQP, aquaporins.
DISCUSSION
Investigating the AQP proteins expressed in the testes, and determining their
localization in the target cells will help to predict and understand their specific
roles in the central processes of fluid secretion and absorption which are mainly
involved in spermatogenesis, sperm transition, and sperm maturation. Herein, our
results provided a comprehensive description of the expression and localization
patterns of different AQP subtypes in the adult mouse testes and testicular
spermatozoa. It is noteworthy that the presence of AQP channels in the germ cells is
involved, in somehow, in the rapid reduction in germ cells volume during
spermatogenesis (Kageyama et al., 20001) due to the high osmolarity of the
seminiferous tubules (Levine & Marsh
1971), and later participating in the sperm maturation and function
(Chen et al., 2011; Squillacioti et al., 2021). AQPs may also be
involved as one of the mechanisms facilitating the function of Leydig and Sertoli
cells to regulate spermatogenesis via secretion and transport of the related
hormones. Moreover, in Sertoli cells, AQPs may facilitate nutrients and fluid
secretion to support germ cells nutrition as well as facilitate sperm transition
through the lumen of seminiferous tubules (Nihei
et al., 2001; Rato et al.,
2010).Among five AQP subtypes that were tested in the present study, AQP7 was the most
abundant AQP protein expressed in the mouse testes. This finding was in accordance
with those of Bernardino et al. (2018) who
reported the intense expression of AQP7 at mRNA level in mouse testes using qPCR
assay, and this expression was higher than those of AQP3 and AQP9. Herein, AQP7 was
strongly expressed and observed in the germinal epithelium and Leydig cells, as well
as overall the testicular spermatozoa. Surprisingly, these findings were not largely
in accordance with those previously reported in humans (Yeung et al., 2009; Moretti
et al., 2012; Laforenza et al.,
2017), boar (Prieto-Marínez et
al., 2016; Vicente-Carrillo et al.,
2016), rat (Calamita et al.,
2001a, 2001b; Hermo & Smith 2011), or even mouse
(Skowronski et al., 2007); they
reported the exclusive presence of AQP7 only in the round and/or elongated spermatid
as well as in secondary spermatocytes in some rat strains (Kageyamaet al., 2001). Moreover, they also reported variable
localization patterns of AQP7 in the sperm cells among the different species; the
differences were also reported in the same species in the different studies.
Notably, Calamita et al. (2001b) suggested
that the possibility of a strain-to-strain and species-to-species variability should
not be overlooked when comparing the AQPs expression.Regarding AQP3, its expression in the mouse testes was not strong as AQP7; in spit of
their localization was more similar. Like our findings, not strong expression of
AQP3 was observed in the mouse testes at the mRNA level (Ma et al., 2000; Bernardino
et al., 2018). Also, the localization of AQP3 in mouse testes in the
present study was more similar to those observed in dog testes (Mirabella et al., 2021) and mouse sperm
(Chen et al., 2011). Interestingly,
although the expression of AQP7 in the mouse testes in this study was more abundant
and stronger than those of AQP3 and according to the correlation between AQP7
expression and lower sperm motility as mentioned before, but we can suggest that
AQP3 is more important for male reproduction, and AQP7 function during
spermatogenesis is not indispensable and can be compensated by another AQPs or other
different mechanisms. This suggestion is based on the findings that; the AQP7
knockout mouse was fertile with normal sperm concentration and morphology (Sohara et al., 2007). In contrast, Chen et al. (2011) reported the subfertility
of AQP3 knockout mice and suggested that AQP3 is an essential membrane pathway
optimizing postcopulatory sperm behavior.Regarding AQP8, its expression was observed only in spermatogonium and Leydig cells.
Surprisingly, several contradicted results have been published regarding the
expression and localization of AQP8 in the rat testes and testicular sperm (Calamita et al., 2001a, 2001b; Elkjær et
al., 2001; Tani et al., 2001;
Badran & Hermo 2002; Yeung et al., 2009). However, to the best of
our knowledge, this is the first report about the expression of AQP8 in Ledyig cells
in mouse testes. Moreover, the expression of AQP9 in the present study was observed
as a strong expression in tails of elongated spermatids and spermatozoa and weak
expression in basal and adluminal and interstitial compartments of seminiferous
tubules. Similar to our findings, AQP9 has been reported to be localized on boar
sperm tail (Vicente-Carrillo et al., 2016),
however, it has no specific staining pattern in human sperm (Yeung et al., 2009). Furthermore, except for the finding of
Domeniconi et al. (2007) who reported
that AQP9 is not expressed in the dog testes, many other authors reported the
expression of AQP9 in the Leydig cells in humans (Arena et al., 2011), and rats (Elkjær et al., 2000; Nicchia et
al., 2001; Badran & Hermo,
2002). According to these findings and ours, it seems that AQP9 is a
common AQP in Leydig cells in humans and rodents. The presence of different AQP
subtypes in the Leydig cells may suggest them as one of the mechanisms facilitating
the endocrine function of Leydig cells to regulate spermatogenesis via secretion and
transport the related hormones, as previously reported in the case of pituitary
endocrine cells (Arnaoutova et al., 2008).
Moreover, the presence of AQP8 and AQP9 on testicular spermatozoa may also suggest
their involvement in sperm function. However, it seems that AQP8 is not
indispensable for male fertility, because Yang et
al. (2005) reported that the AQP8-knockout mice did not show impaired
fertility or abnormalities in sperm count or morphology. Altogether, the abundant
expression of the different AQPs in the male reproductive tissues and the fertility
of AQPs knock-out mice may suggest that the AQPs are important proteins in the male
reproduction, however the functional loss of one AQP subtype in the knock-out mice
may be compensated by the other AQPs; especially when considering the fact that
there are different AQP subtypes which have similar functions.Finally, AQP1 expression in the testes was the weakest among the AQP subtypes tested.
Lower expression of AQP1 was also previously observed in mouse testes at mRNA and
protein levels using qPCR and Western blotting assays, but not using
immunohistochemistry assay (Danyu et al.,
2008; Lu et a., 2008). However,
using immunofluorescence assay in the present study we could detect weak signals of
the labeled antibody against AQP1 in the testes which may indicate to the higher
sensitivity and specificity of the antibody used in the present study.In summary, using the immunofluorescence assay in the present study allowed us to
detect the high variation among the tested AQP protein subtypes regarding their
expression and localization patterns in the mouse testes and testicular spermatozoa.
Moreover, it is allowed to detect that some AQP subtypes are expressed and localized
in the mouse testes and testicular spermatozoa with a specific patterns different
than those previously reported in different mammalian species or even different
mouse strains. Although some available data concerning some AQP subtypes were not
consistent with our findings or even scarce. However, it seems that the AQPs
expression and localization in the male testes and testicular spermatozoa is
species/strain specific. On the other hand, the abundant expression of AQPs in the
testes suggested that the AQPs are indispensable for male reproductive physiology.
Meanwhile, these AQPs are working concurrently and the defect/loss of any AQP
subtype may compensate for the other AQP subtypes. This suggestion is based on the
fact that the AQP knockout mice are not sterile. Finally, further experiments
investigating the detailed expression and localization of the different AQPs along
the male reproductive organs in the different mammalian species are required to
fully understand the role of these proteins in male fertility.
Authors: N Pastor-Soler; C Bagnis; I Sabolic; R Tyszkowski; M McKee; A Van Hoek; S Breton; D Brown Journal: Biol Reprod Date: 2001-08 Impact factor: 4.285
Authors: Raquel L Bernardino; David F Carrageta; Ana M Silva; Giuseppe Calamita; Marco G Alves; Graça Soveral; Pedro F Oliveira Journal: Cells Date: 2018-09-28 Impact factor: 6.600
Fig. 1.
Fig. 2.
Fig. 3.
Fig. 4.