Sung Woo Kim1, Bongki Kim2. 1. Animal Genetic Resource Research Center, National Institute of Animal Science, Hamyang 50000, Korea. 2. Department of Animal Resources Science, Kongju National University, Yesan 32439, Korea.
The epididymis is a critical organ in the male reproductive tract where immature
spermatozoa go through several maturation processes and mature spermatozoa are
stored before ejaculation. The epididymis is structured by a highly convoluted
tubule and is separated into three distinct regions, namely, the caput, corpus, and
cauda epididymis, based on their morphology, histology, physiology, and function
[1,2]. The spermatozoon produced in the testis is transcriptionally and
translationally silent and lacks fertility ability [3]. Therefore, this cell must undertake post-testicular maturation steps
by traveling through the entire epididymal lumen, which is arranged with the
pseudostratified columnar epithelium [4-9]. The epididymal
epithelium comprises a few different cell types including principal cells (PCs),
clear cells (CCs), narrow cells (NCs), and basal cells (BCs). Various proteins that
are produced and released from these major cell types can regulate and create a
special luminal condition that is attributed to sperm maturation and acts as a
reservoir in the epididymis [10-14].NCs and CCs express high levels of vacuolar ATPase (V-ATPase) in their apical
membranes and are required for the formation of an acidic luminal pH that provides
to sustain spermatozoa in a deactivated status during their maturation and storage
in the epididymis. These two cell types are important for luminal acidification of
the epididymis; yet, they are present in very different distributions along the
epididymis. NCs are comparatively small in number and are situated only in the
initial segments. CCs are widely distributed in the caput, corpus, and cauda
epididymis and dramatically increase in number from the proximal to the distal
regions [14,15]. The morphological characteristics of CCs differ depending on the
regions of the epididymis where they are found. For example, CCs are bowl and
cuboidal-shaped in the caput/corpus and cauda, respectively, in mice [16]. Recently, we reported that bowl-shaped CCs
are only pertained in the epididymis of bats [17], whereas, in pigs, bowl-shaped CCs are only located in the caput
regions and are absent in other regions of the epididymis [18]. Therefore, the distribution and localization of CCs show
species-specific patterns. In addition, recent study has reported that a loss of CCs
can lead to elevation of luminal pH in the epididymis and result in decreased sperm
fertility [19]. BCs display a hemispherical
morphology and are placed underneath other epithelial cells and are in contact with
the basement membrane. Recently, however, it was observed that BCs appear in
different morphological features in the epithelium of the epididymis and trachea.
They can extend their long and narrow projections, cross tight junctions, and scan
luminal environments in rodents [20,21]. In addition to luminal acidification, BCs
are an indirect player in regulating luminal pH via communication with CCs in the
rat epididymis [22]. Therefore, the
interactions between these two cell types, CCs and BCs, is necessary to create an
ideal luminal condition for maturation and storage processes of spermatozoa.
However, limited knowledge exists regarding the regulation and establishment
mechanisms of the optimal luminal environment in the epididymis of bulls. To improve
our understanding of these mechanisms, more studies related to the localization and
distribution of these epididymal epithelial cells are required.Here, we examined the presence and distribution of the B1 subunit of V-ATPase
(B1-VATPase) and cytokeratin 5 (KRT5) (also known as CC and BC markers,
respectively) in the bovine epididymis. Determining the specific distribution of
epididymal epithelial cells may help understand the regulatory system to create a
perfect internal milieu for maturation and storage of spermatozoa in the bovine
epididymis. As far as we know, this study is the first to apply immunohistochemical
markers to investigate their expression and localization into epithelial cells and
spermatozoa of the adult bovine epididymis.
MATERIALS AND METHODS
Animals and ethics statement
Five bulls between 26 and 28 months of age were used for this experiment. The
epididymides were collected from a local slaughterhouse (Yesan, Chungnam,
Korea). All animal procedures used in this study were approved by the Animal
Care and Use Committee of the National Institute of Animal Science (NIAS
2018-290).
Tissue fixation and preparation
The bovine epididymides were dissected and immediately placed in 4%
paraformaldehyde (4% PFA) for 48 h at room temperature (4% PFA was replaced with
fresh fixative every 12 hours), followed by three × 15-min washes in PBS.
The tissues were transferred to 30% sucrose solution in PBS until the tissues
sink to the bottom of the containers. The tissues were then placed in OCT
compound (Thermo Scientific, Rockford, IL, USA), embedded in molds, and frozen
with dry ice. The tissues were cut at 10 µm using a Leica 3050S cryostat
(Leica Biosystems, Wetzlar, Germany), placed onto Muto New Silane III coating
slides (Muto Pure Chemical, Tokyo, Japan), and stored at −80°C
until subsequent use. For histological observation, hematoxylin and eosin
(H&E) staining was performed as described before [23].
Immunofluorescence staining and antibodies
The sections were thawed at room temperature for 10 min, and rehydrated in PBS
for 10 min. To unmask antigens, the slides were placed in a microwave-resistant
jar containing an alkaline buffer (Vector Laboratories, Burlingame, CA, USA) and
microwaving for 2 min on high power (repeat three times with 5-min intervals
between steps). After antigen retrieval, the slides were allowed to cool slowly
to room temperature for at least 30 min. The slides were then washed three times
with PBS and were incubated with the blocker solution (Thermo Scientific) to
block non-specific antibody binding for 30 min at room temperature. The slides
were then incubated with the primary antibodies. After some washing steps,
secondary antibodies were applied. The slides were rinsed between antibody
treatments with PBS containing 0.1% Tween-20 (Sigma-Aldrich, St. Louis, MO,
USA). The incubation times of primary and secondary antibodies vary from 60 min
at room temperature to overnight at 4°C. The slides then counterstained
and mounted with Vectashield antifade mounting medium (Vector Laboratories)
containing 4′,6-diamidino-2-phenylindole (DAPI). Coverslips were sealed
with clear nail polish. To observe CCs and BCs, the slides were stained with a
chicken polyclonal antibody against the B1-VATPase (diluted 1:1,500) [18] and a rabbit polyclonal antibody
against the KRT5 (diluted 1:300; Thermo Scientific) [21], respectively. For the co-localization studies, primary
and secondary antibodies were applied sequentially, as described above. The
following all secondary antibodies used in this experiment were purchased from
Jackson ImmunoResearch Laboratories (West Grove, PA, USA): Cy3-conjugated donkey
anti-chicken IgG (1:600) and Alex Fluor®488-conjugated donkey anti-rabbit
IgG (1:300). Dako antibody diluent (DAKO, Carpinteria, CA, USA) was used for
dilution of primary and secondary antibodies. For negative control, the same
staining protocol without the addition of primary antibodies was performed. The
slides were observed under an LSM800 confocal microscope (Carl Zeiss, Jena,
Germany) and acquired confocal images were analyzed using Zen Blue (Lite)
software.
Quantification of clear and basal cells
B1-VATPase and KRT5 antibodies were used to perform immunofluorescence staining
of CCs and BCs, respectively. At least three epididymides obtained from
different individual males were examined. The numbers of CCs and BCs were
measured by manually counting the number of B1-VATPase- and KRT5-positive cells
per square millimeter epithelium area. To measure B1-VATPase-positive BCs,
double labeled epithelial cells were also examined as described above. Zeiss
confocal microscope was used to acquire digital images (20×
objective).
Protein extraction and immunoblotting
Tissues were lysed for 30 min on ice in RIPA buffer (Thermo Scientific)
containing complete protease inhibitors and phosphatase inhibitors (Roche
Applied Science, Indianapolis, IN, USA). The lysate was centrifuged at
16,000×g for 30 min at 4°C and the supernatant was collected. For
electrophoresis, samples were prepared in LDS Sample Buffer (Invitrogen) with 4%
b-mercaptoethanol and incubated for 30 min at room temperature. The protein was
loaded on LDS polyacrylamide gel and electrophoresed as described before [24]. The separated proteins were
transferred onto Immun-Blot polyvinylidene difluoride (PVDF) membranes.
Antibodies against B1-VATPase (diluted 1:2,500), and KRT5 (diluted 1:1,000) were
used and the labelled antigens were detected by chemiluminescence and Kodak
imaging films.
Statistical analysis
The epididymides from at least three bulls were used for all experiments, and for
each epididymis, three sections were examined. The numbers of CCs and BCs were
analyzed using one-way analysis of variance (ANOVA) test and the significant
difference between means of analyzed data was analyzed using Duncan’s
multiple range test. A significant difference was indicated by
p < 0.01. Measurements of the epithelial area were
performed by using Zen Blue (Lite) software.
RESULTS
Expression and localization of B1-VAPTase in the adult bovine
epididymis
In the present study, the epididymis of bulls was labeled to examine the presence
and localization of B1-VATPase. As shown in Fig.
1, B1-VATPase was expressed and localized in two different cell
types, with both cell types lying on the epithelium. Epithelial cells with
nuclei positioned close to the lumen were observed with a narrow-shaped
morphological characteristic (Fig. 1,
arrows) and the other type of epithelial cells was located beneath the basal
lamina where BCs were commonly present (Fig.
1, arrowheads). Specialized cells with high expression of V-ATPase in
their apical membrane and the nucleus adjacent to the luminal aspect are
classical characteristics of epididymal CCs in many species, e.g., mice, rats,
pigs, and bats. Therefore, we called these specialized cells narrow-shaped CCs.
These narrow-shaped CCs were present from the caput to the corpus; however, they
were disappeared in the cauda regions of the epididymis (Fig. 1). The number of cells was much less in the corpus
than that in the caput (Fig. 2A). On the
other hand, V-ATPase positive cells located in the lower parts of the epithelium
were observed in all epididymal regions from the caput and cauda (Fig. 1, arrowheads). The number of V-ATPase
positive cells located in the lower parts of the epithelium was highest in the
corpus, followed by the caput and cauda epididymal segments (Fig. 2B). V-ATPase-positive spermatozoa were
observed in the corpus and cauda (Fig. 1,
yellow arrowheads) but not in the caput epididymis (Fig. 1). No labeling was detected from negative controls
(Supplementary Fig. S1A and D). Western blotting confirmed the expression of
B1-VATPase in the bovine epididymis (Supplementary Fig. 1G).
Fig. 1.
Localization of B1-VATPase in the adult bovine epididymis.
White arrows indicate narrow shaped-CCs and white arrowheads indicate
B1-VATPase positive cells located beneath the basal lamina. Yellow
arrowheads indicate B1-VATPase positive-spermatozoa. Zoomed-in views of
the white and yellow dashed boxes are shown in the rightmost panel of
each lane and delineate epithelial cells and spermatozoa, respectively.
S, spermatozoa. Nuclei counterstaining was carried out by DAPI (blue).
Scale bar = 20 µm. B1-VATPase, B1 subunit of V-ATPase; CCs, clear
cells; DAPI, 4′,6-diamidino-2-phenylindole
Fig. 2.
Quantitative analysis of the distribution of the various cell types
along the epididymis.
(A) Narrow-shaped CCs, (B) B1-VATPase positive BCs, and (C) KRT5 positive
BCs were counted in each region of the epididymis. Cell numbers were
obtained from the number of B1-VATPase, KRT5, or both positive cells in
the caput, corpus, and cauda, and normalized to per square millimeter of
the epithelium area. Results are expressed as the mean ± SEM.
Different numbers represent significant differences among groups
(p < 0.01). CCs, clear cells; B1-VATPase, B1
subunit of V-ATPase; BCs, basal cells; KRT5, cytokeratin 5.
Localization of B1-VATPase in the adult bovine epididymis.
White arrows indicate narrow shaped-CCs and white arrowheads indicate
B1-VATPase positive cells located beneath the basal lamina. Yellow
arrowheads indicate B1-VATPase positive-spermatozoa. Zoomed-in views of
the white and yellow dashed boxes are shown in the rightmost panel of
each lane and delineate epithelial cells and spermatozoa, respectively.
S, spermatozoa. Nuclei counterstaining was carried out by DAPI (blue).
Scale bar = 20 µm. B1-VATPase, B1 subunit of V-ATPase; CCs, clear
cells; DAPI, 4′,6-diamidino-2-phenylindole
Quantitative analysis of the distribution of the various cell types
along the epididymis.
(A) Narrow-shaped CCs, (B) B1-VATPase positive BCs, and (C) KRT5 positive
BCs were counted in each region of the epididymis. Cell numbers were
obtained from the number of B1-VATPase, KRT5, or both positive cells in
the caput, corpus, and cauda, and normalized to per square millimeter of
the epithelium area. Results are expressed as the mean ± SEM.
Different numbers represent significant differences among groups
(p < 0.01). CCs, clear cells; B1-VATPase, B1
subunit of V-ATPase; BCs, basal cells; KRT5, cytokeratin 5.
Expression and localization of KRT5 in the adult bovine epididymis
The KRT5 antibody was used as a marker of BCs in the epididymis. KRT5 positive
cells were present in the base of the epithelium and had a dome-shaped
morphology from all regions of the epididymis (Fig. 3). No axopodia cells displaying a long cytoplasmic projection
were present in any regions of the epididymis. No KRT5 expressed spermatozoa
were detected in the epididymis. The largest number of BCs was observed in the
corpus, followed by the caput and cauda (Fig.
2C). No labeling was detected from negative controls (Supplementary
Fig. 1B and E). Western blotting confirmed the expression of KRT5 in the bovine
epididymis (Supplementary Fig. 1G).
Fig. 3.
Localization of KRT5 in the adult bovine epididymis.
Arrowheads indicate KRT5 positive epithelial cells. KRT5 positive cells,
BCs are only present in the base of the epithelium from all regions of
the epididymis. Zoomed-in views of the dashed boxes are shown in the
rightmost panel of each lane. Nuclei counterstaining was carried out by
DAPI (blue). Scale bar = 20 µm. KRT5, cytokeratin 5; BCs, basal
cells; DAPI, 4′,6-diamidino-2-phenylindole.
Localization of KRT5 in the adult bovine epididymis.
Arrowheads indicate KRT5 positive epithelial cells. KRT5 positive cells,
BCs are only present in the base of the epithelium from all regions of
the epididymis. Zoomed-in views of the dashed boxes are shown in the
rightmost panel of each lane. Nuclei counterstaining was carried out by
DAPI (blue). Scale bar = 20 µm. KRT5, cytokeratin 5; BCs, basal
cells; DAPI, 4′,6-diamidino-2-phenylindole.
Colocalization of B1-VATPase and KRT5 in the adult bovine epididymis
To confirm whether V-ATPase was expressed in the BCs, B1-VATPase and KRT5 were
double-labeled in the bovine epididymis. B1-VATPase was clearly expressed in two
different localizations in both the caput and corpus (Fig. 4, white arrows and red arrowheads), whereas KRT5 was
only present at the lower part of the epithelium from all regions of the
epididymis (Fig. 4, green arrowheads).
Epithelial Cells co-labeled with B1-VATPase and KRT5 antibodies were detected in
the lower part of the epithelium from the caput to the cauda regions of the
epididymis (Fig. 4, yellow arrowheads).
Only B1-VATPase positive cells (narrow-shaped CCs) were detected in the caput
and corpus (Fig. 4G and H, arrows). Thus, V-ATPase was expressed in
BCs as well as in CCs in the bovine epididymis. No labeling was detected from
negative controls (Supplementary Fig. 1C, and F). Histological analysis revealed
that the epididymal epithelium is pseudostratified and contains CCs and BCs with
different locations (Supplementary Fig. S1H-M).
Fig. 4.
Colocalization of B1-VATPase and KRT5 in basal cells of the bovine
epididymis.
Representative images for double immunofluorescence labeling of
B1-VATPase (red) and KRT5 (green). White arrows indicate narrow
shaped-CCs in the epithelium. Red, green, and yellow arrowheads indicate
B1-VATPase, KRT5, and both antibodies positive cells, respectively.
Zoomed-in views of the dashed boxes are shown in the rightmost panel of
each lane. Nuclei counterstaining was carried out by DAPI (blue). Scale
bar = 20 µm. B1-VATPase, B1 subunit of V-ATPase; KRT5,
cytokeratin 5; CCs, clear cells; DAPI,
4′,6-diamidino-2-phenylindole.
Colocalization of B1-VATPase and KRT5 in basal cells of the bovine
epididymis.
Representative images for double immunofluorescence labeling of
B1-VATPase (red) and KRT5 (green). White arrows indicate narrow
shaped-CCs in the epithelium. Red, green, and yellow arrowheads indicate
B1-VATPase, KRT5, and both antibodies positive cells, respectively.
Zoomed-in views of the dashed boxes are shown in the rightmost panel of
each lane. Nuclei counterstaining was carried out by DAPI (blue). Scale
bar = 20 µm. B1-VATPase, B1 subunit of V-ATPase; KRT5,
cytokeratin 5; CCs, clear cells; DAPI,
4′,6-diamidino-2-phenylindole.
DISCUSSION
V-ATPase and KRT5 have been used as CC and BC markers, respectively, in many species
including mice, rats, pigs, and bats. We first observed the expression and
localization of CCs and BCs using B1-VATPase and KRT5 antibodies in the adult bovine
epididymis. BCs were maintained in all portions of the epididymis and had a
dome-shaped morphology. This result is in agreement with earlier researches in pigs
and bats that do not have any projected BCs but have only dome-shaped BCs [17,18].
In rodents, however, the BCs were present with region-specific morphological
characteristics. For example, the observation of BCs with long and narrow
projections were confirmed in the initial segment and distal corpus/proximal cauda
in mice [21] and rats [22], respectively. Thus, the morphological characteristics of
the epididymal BCs are species-specific. In this study, we suggested that CCs were
observed with a narrow-shaped morphology from the caput to the corpus; however, they
were not present in the cauda region of the epididymis. Earlier studies have
reported that CCs are localized differently depending on the species. In pigs, CCs
were only localized in the caput region [18],
but CCs in bats have been observed in all regions of the epididymis [17]. Regarding the morphological features of
CCs, bowl-shaped CCs were observed in pigs and bats [17, 18]; however, in mice, the
CCs were shown with various morphologies such as narrow-, bowl-, and cuboidal-shaped
morphologies in their regions of the epididymis [15]. Thus, CCs have species/region-specific distribution and morphology.
In the present study, both B1-VATPase and KRT5 were co-expressed in the BCs of the
adult bovine epididymis. This observation is consistent with our goat study where
B1-VATPase and KRT5 were co-localized in adult goat epididymis but not before
puberty [25]. According to previous studies,
however, B1-VATPase and KRT5 were not co-expressed and co-localized in the
epididymal epithelium in pigs, mice, rats, and bats [15,17,18,26]. Therefore, these
co-localization patterns of V-ATPase and KRT5 in BCs could be specific to ruminant
animals.The V-ATPase is confined to the apical membranes of CCs of the epididymis and is a
major contributor to luminal acidification by secreting protons into the epididymal
luminal. Recent studies on the epididymis have shown an elaborate communication
network exists between CCs and BCs, and between CCs and PCs, to establish and
maintain luminal acidification that is necessary for sperm maturation and storage
[22,27]. The pH in bovinecauda epididymis was reported to be approximately
6.8 by Wales et al. [28] and approximately
5.8 as reported by Acott and Carr [29]. These
acidic conditions in the epididymis could be controlled by epithelial cells and
other cells. No CCs were present in the cauda epididymis in the present study;
rather, BCs expressed B1-VATPase. However, we still have insufficient data to
interpret the acidification mechanism of the bovinecauda epididymis. The mechanism
could be complicatedly regulated by many factors. We speculate that in the bovine
epididymis, there are two hypotheses for maintaining the acidic luminal condition:
1) V-ATPase-positive BCs might directly secrete protons into the lumen and 2) PCs
might secrete less HCO3− to alleviate luminal pH in the
bovine epididymis. Additional researches are required to elucidate the fundamental
mechanisms for the establishment and regulation of luminal acidification in the
bovine epididymis.Here, we report that V-ATPase was highly expressed in the cauda spermatozoa but less
expressed in the caput spermatozoa. These results are in agreement with a previous
study that the a2 isoform of V-ATPase (ATP6V0A2) was highly expressed in normal
human spermatozoa (motile) but was not detected in spermatozoa (immotile) from
infertile men [30]. The epididymal transit
from the caput to the cauda is necessary for sperm maturation, the acquisition of
motility, and the ability to fertilize eggs. Therefore, V-ATPase in bovine
spermatozoa may be a vital molecule for controlling sperm maturation and could be
used as a biomarker candidate for the evaluation of bull infertility in the AI
center.In conclusion, B1-VATPase is expressed in CCs, BCs, and cauda spermatozoa in the
bovine epididymis. These highly specific expression patterns in the bovine
epididymis might be important for the establishment and maintenance of an ideal
internal environment for the maturation and storage of spermatozoa. However, to
identify a novel function of V-ATPase to regulate the unique luminal environment in
the bovine epididymis, it is essential to increase our understanding of the
regulatory mechanism by systemic cell-cell communications and intense cell-sperm
interactions.
SUPPLEMENTARY MATERIALS
Supplementary Materials Are Only available online from: https://doi.org/10.5187/jast.2021.e32.
Authors: Dario Krapf; Ye Chun Ruan; Eva V Wertheimer; Maria A Battistone; John B Pawlak; Archana Sanjay; Stephen H Pilder; Patricia Cuasnicu; Sylvie Breton; Pablo E Visconti Journal: Dev Biol Date: 2012-06-30 Impact factor: 3.582
Authors: Carmen Díez-Sánchez; Eduardo Ruiz-Pesini; Julio Montoya; Acisclo Pérez-Martos; José Antonio Enríquez; Manuel J López-Pérez Journal: FEBS Lett Date: 2003-10-09 Impact factor: 4.124
Fig. 1.
Fig. 2.
Fig. 3.
Fig. 4.