ARTICLE |
Correspondence to: Gustavo Blanco, Dept. of Cell Biology and Physiology, Washington U. School of Medicine, 660 S. Euclid Avenue, St Louis, MO 63110. E-mail: gblanco@cellbio.wustl.edu
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Summary |
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In addition to the three isoforms of the catalytic subunit of the Na,K-ATPase originally identified (1,
2, and
3), a fourth
polypeptide (
4) has recently been found in mammalian cells. This novel
-subunit of the Na,K-ATPase is selectively expressed in male gonadal tissues. In the testes,
4 is functionally active and comprises approximately half of the Na,K-ATPase activity of the organ. At present, the pattern of expression of the
4 polypeptide within the cells of the male gonad is unknown. By in situ hybridization, immunocytochemistry, and the ouabain inhibition profile of Na,K-ATPase activity, we show that the
4-subunit is expressed in the germ cells of rat testes. The highest amounts of the isoform are found in spermatozoa, where it constitutes two thirds of the Na,K-ATPase activity of the gametes. The other Na pump present in the cells is the ubiquitously expressed
1 polypeptide. The characteristic localization of
4 in the gonad is further supported by the drastic reduction of the polypeptide in mice that are infertile as a consequence of arrest in maturation of the germ cells. In addition, GC-1spg cells, a murine cell line derived from testis spermatogonia, also contain the Na,K-ATPase
4 polypeptide. However, the level of expression of the isoform in these cells is much lower than in the spermatozoa, a fact that may depend on the limited ability of the GC-1spg cells to differentiate in vitro. The particular expression of the Na,K-ATPase
4 isoform we encounter and the specific enzymatic properties of the polypeptide suggests its importance for ionic homeostasis of the germ cells of the testes. (J Histochem Cytochem 48:10231032, 2000)
Key Words:
Na,K-ATPase, isozymes, 4 isoform, testes, spermatozoa
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Introduction |
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The Na,K-ATPase or Na pump exists as multiple isozymes consisting of different - and ß-subunits (reviewed in
-subunits (
1,
2,
3, and
4) and three different ß-subunits (ß1, ß2, and ß3) have been identified in vertebrates (
and ß polypeptides and their ability to associate in different pairs provides each cell with a particular array of Na,K-ATPase isozymes (reviewed in
ß complexes (
4-subunit. Recently, studies of the function of this polypeptide have confirmed that it can function as a catalytic subunit of the Na,K-ATPase. Thus, the
4 isoform is able to bind [3H]-ouabain, become phosphorylated from ATP, hydrolyze ATP, and transport 86Rb, in a manner typical for a Na,K-ATPase (
isoform,
4, exhibits enzymatic characteristics that distinguish it from the other
isoforms. For example,
4 is very sensitive to ouabain, has a high apparent affinity for Na+, a low affinity for K+, and an intermediate affinity for ATP (
4 polypeptide is its limited tissue localization. The isoform appears to be selectively expressed in the testes and epididymis (
1 and
4 isoforms (
4 isoform in the physiology of the testes is unknown. An important goal in understanding the role of this isoform is to determine the distribution of the polypeptide within the cells of the gonad. On the basis of in situ hybridization analysis, immunocytochemistry, and the ouabain inhibition profiles of the Na,K-ATPase activity, we present evidence that, in the testes, the
4 polypeptide is expressed in the germ cells and predominantly in spermatozoa.
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Materials and Methods |
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Tissue and Cells
Testes and sperm cells or the germ cell line GC-1spg were used in this study. Testes were obtained from adult SpragueDawley rats weighing 200240 g or from adult mice. In the case of mice, normal and transgenic mice deficient in the translation factor Egr4 (
Tissue and Cell Preparations
Membrane fractions were prepared from adult rat and mouse testes according to the protocol described previously (
RNA Blotting Analysis
RNA was isolated from tissue and cells using RNAzol according to the suppliers protocol (Tel-Test; Friendswood, TX). RNA content was quantified spectrophotometrically. Equal amounts of RNA (15 µg) were separated by electrophoresis in a formaldehyde gel and transferred overnight by capillary action to nitrocellulose (Micron Separations; Westboro, MA). The blots were UV-crosslinked and prehybridized at 65C according to isoforms were made from N-terminal fragments of the corresponding cDNAs, using the Rediprime random primer labeling kit from Amersham (Poole, UK). For the
1 and
3 isoforms, a cDNA segment corresponding to the 5' end of each isoform to the AflII restriction site was used as template. For
2, a region of the isoform spanning from the 5' end to the NheI site was used. For
4, the segment between base pairs 1314 and 1592 was utilized. Blots were washed in 0.1 x SSC (15 mM NaCl, 0.15 mM sodium citrate, pH 7.0), containing 1% SDS at 65C and exposed for autoradiography.
In Situ Hybridization
Localization of the Na,K-ATPase 4 isoform RNA was performed on 10-µm-thick sections of rat testes that had been fixed in 2% paraformaldehyde and embedded in paraffin. In situ hybridization was performed using the RNA Colour kit from Amersham. The fluorescein11-UTP-labeled probes for the
1 and
4 isoforms were made using as template the full-length cDNA for the
1-subunit or a 301-bp cDNA fragment (bases 13141592 of the coding region of
4) for the
4-subunit. Transcription from both
isoform cDNAs, subcloned into pGEM-T Easy vector (Promega; Madison, WI) was performed using SP6 RNA polymerase. Sense probes using as template the same
1 and
4 cDNAs were made and used as control. Hybridization with the probes was performed for 2 hr at 55C. Samples were washed twice for 10 min each with 0.1% (v/v) of sodium dodecyl sulfate (SDS) in SSC at room temperature (RT), followed by two other washes at 55C for 10 min with 0.1% (v/v) SDS in SSC. The labeled probes were detected using an anti-fluorescein antibody conjugated to alkaline phosphatase at a dilution of 1:100.
Immunocytochemistry
Paraffin sections (10 µm) of rat testes, were treated with xylene and ethanol to remove the paraffin. After hydration, permeabilization of the sections was achieved by a 15-min incubation at 25C with 0.3% Triton X100 in HBS (25 mM Hepes, pH 7.4, 150 mM NaCl, and 1 mM EGTA). The tissue was then blocked for 2 hr at RT in 0.2% BSA, 5% normal goat serum (NGS) in HBS. The primary antibody in HBS containing 0.1% BSA, 2% NGS was added and allowed to attach overnight at 4C. After three 5-min washes in HBS, the secondary antibody in HBS containing 0.1% BSA, 2% NGS was added. After 1 hr, sections were washed three times for 5 min each with HBS and mounted. The 1 polypeptide was detected with a 1:100 dilution of an antiserum that recognizes a N-terminal peptide (DKYEPAAVSEHGD) of the isoform (
4 isoform, a specific antiserum against a peptide (SEQKPRPTLRASNTNRQPK) corresponding to a sequence at the N-terminus of the
4 polypeptide was used at a dilution of 1:100 (
Biochemical Assays
Protein assays were performed using the bicinchoninic acid/copper sulfate solution as described by the supplier (Pierce Chemical; Rockford, IL) after lysis of the cells in 1% 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS). Na,K-ATPase activity was assayed through determination of the initial rate of release of 32Pi from [32P]-ATP as described previously (
[32P]-ATP ± different concentrations of ouabain. The reaction was started by the addition of ATP and incubated at 37C for 30 min. Radioactivity of 170 µl of the isobutanol-phosphomolybdate phase was measured by liquid scintillation counting. The hydrolysis of ATP in all assays was linear over the time course of the reaction. The total hydrolysis of ATP among the various preparations ranged from 30 to 50 µmoles of Pi released/mg protein/hr. Specific Na,K-ATPase activity was approximately 3 and 7 µmoles of Pi released/mg protein/hr for the Na,K-ATPase from rat and mouse testes, respectively. The germ cell line in culture and the spermatozoa showed lower specific activity, with values of approximately 1 and 2 µmoles of Pi released/mg protein/hr, respectively. Na,K-ATPase activity was determined as the hydrolysis of ATP that was dependent on Na+ and K+ and sensitive to 1 mM ouabain. Thus, total Na,K-ATPase activity was calculated by subtracting the ATPase activity obtained in the presence of 1 mM ouabain from that measured in its absence. For the ouabain doseresponse curves, activity values were standardized to compare the relative contribution of each Na,K-ATPase isozyme to the total activity of each sample. For this, data were expressed as a percentage of the total Na,K-ATPase sensitive to 1 mM ouabain.
Data Analysis
Curve fitting of the experimental data was performed using a Marquardt least-squares nonlinear regression computing program (Sigma Plot; Jandel Scientific, San Rafael, CA). Doseresponse relations for the ouabain inhibition of Na,K-ATPase activity showed a heterogeneous population of enzyme that was best fitted by applying an equation that assumed the existence of two (Equation 1) populations of Na,K-ATPase isozymes with different affinities for ouabain:
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(1) |
where v is the Na,K-ATPase activity corresponding to a certain concentration of the inhibitor ouabain [I], expressed as a fraction of activity in the absence of ouabain. F1 and F2 are the fractional amounts of each Na pump isozyme, whereas Ki and Kii represent the concentration of ouabain that gives the half-maximal inhibition to each of the Na,K-ATPases present in the sample. The best fit of the data to a two, rather than a one or multiple enzyme population model was confirmed by applying an F test as reported previously (1 and
4, were present in the samples.
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Results |
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In the testes, the expression of the -subunit of the Na,K-ATPase has been reported to be limited to the
1 and
4 isoforms (
-subunits, 32P-labeled probes were made using as template isoform-specific cDNA segments. In addition, hybridization with the probes at 65C and stringent washing conditions using 1% SDS and 0.1% SSC were applied. As shown in Fig 1, transcripts for only the
1- and
4-subunits of the Na,K-ATPase were detected in the testes. As control, total RNA from rat kidney, which contains only the
1 isoform, and brain, which expresses the
1,
2, and
3 isoforms, were used.
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To gain insight into the distribution of the Na,K-ATPase 1 and
4 isoforms in the testes, we determined the localization of the corresponding mRNAs using in situ hybridization. Fluorescein11-UTP-labeled RNA probes, followed by an anti-fluorescein alkaline phosphatase-conjugated antibody, were used to detect the
1 and
4 transcripts. Specific labeling of the isoforms was obtained by hybridization with the probes at 55C and stringent washes. Fig 2 shows that the
1 mRNA was found in the seminiferous tubules as well as at the interstitial cells of the gonad. In contrast, the message for
4 was localized to cells in the pseudostratified epithelium of the seminiferous tubules and mainly at the inner or luminal portions of these structures. The distribution of
4 mRNA is consistent with expression of the isoform in the germ cells. These cells also express the
1 transcript, and there appeared to be no cells that express solely the
4 mRNA. In contrast, cells at the interstitium, between the seminiferous tubules, contain only the RNA for the Na,K-ATPase
1 isoform.
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To investigate the expression of isoforms at the protein level, sections of rat testes were subjected to immunocytochemical analysis using anti-
1 or anti-
4 antibodies, followed by secondary antibodies conjugated to FITC. As shown in Fig 3, a different pattern of distribution of the Na,K-ATPase
1 and
4 polypeptides was found in the gonad. As expected from the expression of the corresponding RNAs, the
1 antiserum evenly labeled all the cells within and between the seminiferous tubules (Fig 3A and Fig 3D), whereas staining with the
4 antiserum showed a more restricted distribution (Fig 3B and Fig 3E). Immunoreactivity for
4 was primarily located on the adluminal side of the seminiferous tubules, with the highest intensity of label found in the spermatozoa. This suggests that the germ cells are the main source of the Na,K-ATPase
4 isoform. However, the polypeptide is not the only Na pump isoform expressed in these cells because
1 was also detected.
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To further study the pattern of expression of the Na,K-ATPase 1 and
4 isoforms in the germ cells of the testis, we determined the profiles of inhibition of Na,K-ATPase activity by ouabain. This approach has been routinely used as a tool to detect Na,K-ATPase isoform content in a sample. The method has the advantage of measuring functionally active Na,K-ATPase molecules and, in addition, it allows a more reliable quantification of the isozymes present (reviewed in
1 and
4 isoforms differ drastically in their affinities for ouabain. Compared to
1, the
4 isoform is over a thousand times more sensitive to the cardiotonic steroid (
isoform to the total Na,K-ATPase of the sample. The functional Na,K-ATPase isoform composition of germ cells was first determined in GC-1spg cells and in spermatozoa. GC-1spg cells are a nontumorigenic murine cell line derived from germ cells of the gonad that have been immortalized by simian virus 40 large tumor antigen transformation (
1 and
4 isoforms (
isoforms in the GC-1spg cells was corroborated by hybridization analysis of total RNA (Fig 4B). As shown, these cells do not express the
2 and
3 isoforms of the enzyme. Therefore, in agreement with the previous results, germ cells express both the
1 and
4 isoforms of the Na,K-ATPase. In addition, the level of isoform activity was unequal, with the
1 isoform making a relatively larger contribution to the total Na,K-ATPase of these cells. Because the turnover number of activity (ATP hydrolysed per min) is similar among the isoforms, their different contribution to the Na,K-ATPase hydrolysis reflect differences in expression of the polypeptides (
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Although the GC-1spg cells have all the characteristics of germ cells, they can differentiate only to a certain extent, reaching a stage between spermatogonia Type B and spermatocytes. To investigate the level of expression of the 4 isoform in fully differentiated germ cells, we studied the profile of ouabain inhibition of the Na,K-ATPase from spermatozoa obtained from rat epididymis. As shown in Fig 5, a biphasic doseresponse curve was found for the interaction of the cardiotonic steroid with the Na,K-ATPase of sperm cells. The obtained Kis for the sensitive and resistant forms of the enzyme corresponded to those of
1 and
4, confirming the expression of both Na pump isoforms in these cells. The calculated Ki and fractional amounts for each isozyme are indicated in Table 1. As shown,
4 activity constitutes the main Na,K-ATPase of spermatozoa. This contrasts with the relative distribution of the isoforms in the cultured germ cells, in which
1 activity represents the predominant Na pump present.
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To further confirm that the expression of the Na,K-ATPase 4 isoform originates mainly from the sperm cells, we characterized the Na,K-ATPase activity in testes from normal mice and mice made infertile through a deficiency in the production of the early growth response transcription factor, Egr4 (
4 isoform is mainly expressed in the mature germ cells, a reduction in the expression of the Na,K-ATPase
4 polypeptide should be expected to accompany the impaired production of spermatozoa in the transgenic mice. Fig 6 shows the ouabain inhibition profiles of the Na,K-ATPase from Egr4-deficient and normal mice testes. Reflecting the presence of both the
1 and
4 isoforms, testes from normal and Egr4-deficient mice exhibited low and high ouabain-sensitive Na,K-ATPase activities. The calculated inhibition constants and relative quantity for the activity of each
isoform are summarized in Table 1. As shown, the normal mice gonad has approximately equal amounts of the
1 and
4 isoforms. This is in agreement with the results from rat testes (
4 isoform and, concomitantly, a proportional increase in the
1 isoform. Taken together, these results indicate that the germ cells express two functionally active isoforms of the catalytic subunit of the Na,K-ATPase,
1 and
4, and that the
4 polypeptide is the main functional form expressed in the meiotic cells of the gonad.
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Discussion |
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The 4 polypeptide is the Na,K-ATPase isoform that exhibits the most restricted pattern of expression, having been solely identified in male gonadal tissues (
4 isoform is not exclusive because the
1 polypeptide is present as well (
2 and
3 isoforms are absent (
1 and
4 isoforms are catalytically functional in the gonad. Although
1 and
4 contribute approximately equally to the Na,K-ATPase activity of the tissue, the isoforms have enzymatic properties that are different (
4 suggest that it performs a specific function. An important goal in understanding the role of
4 is to determine its pattern of expression within the cells of the testes. In the present work we have analyzed this by in situ hybridization, immunocytochemistry, and by the profile of ouabain inhibition. Our results indicate that the
4 isoform is expressed predominantly in differentiated germ cells of the testes.
Although the polypeptide represents the majority of the Na,K-ATPase in the gametes, it is not the only -subunit present because the cells also contain lower amounts of the ubiquitously expressed
1 isoform. The presence of the highly ouabain-sensitive and the ouabain-resistant ATPase activity typical of the
1 and
4 isoforms indicates that both polypeptides are functionally competent in the germ cells. This agrees with previous reports indicating that the meiotic cells of the testes are capable of hydrolyzing ATP in an Na+- and K+-dependent manner (
4 isoform are present in other cells of the testes can not be completely ruled out. For example, the anti-
4 antiserum appears to faintly label the Sertoli cells. However, the level of
4 expression in these cells is sparse. The finding by
1 isoform. In addition, the analysis of the RNA and protein of the Na pump
4 isoform in the space between the seminiferous tubules suggests that the interstitial cells of the testes, such as Leydig cells, express predominantly the
1 isoform. Interestingly, we were unable to identify cells that uniquely express
4. Taken together, these results suggest that the main expression of the Na,K-ATPase
4 polypeptide occurs in the fully mature germ cells. However, the relative levels of activity of the isoform are different when the spermatozoa and the germ cell line GC-1spg are compared. In spermatozoa, the expression of
4 activity clearly predominates over that of the
1 isoform. The opposite occurs in GC-1spg cells, in which the activity of
1 prevails. This dissimilarity in isoform composition between the cultured and native cells may depend on the inability of the GC-1spg cells to fully express the Na,K-ATPase
4 isoform in vitro. This possibility seems unlikely because GC-1spg cells are able to normally express other testis-specific proteins, such as cytochrome ct and the lactate dehydrogenase C4 isozyme (
4 isoform is required at later stages of spermatozoa development. Supporting this notion are the results obtained from testes of Egr4-deficient mice. In these mice, maturation of the germ cells is almost completely blocked at the early-mid pachytene stage of spermatocyte development (
4 isoform is approximately a third of that found in normal testes. This difference, which suggests a developmental modulation of the expression of the Na pump
4-subunit, is not unique for the isoform, because changes in the levels of other Na,K-ATPase
isoforms have been reported during maturation (reviewed in
The high level of expression of the 4 isoform of the Na,K-ATPase in the mature germ cells of testes is intriguing. This occurrence may be related to the particular ionic environment of the germ cells. The medium bathing the cells inside the seminiferous tubules has a concentration of K+ that is higher than that of blood (
4 isoform for K+ is low (
4 isoform function has evolved to adapt to the medium in the tubules. In addition, the increase of
4 in spermatozoa compared to the immature germ cells may be related to the fact that as the cells differentiate they come in contact with the high-K+ fluid in the lumen of the tubules. Another important enzymatic property of the Na,K-ATPase
4 isoform is its high affinity for ouabain. Differences in ouabain sensitivity of the Na,K-ATPase isozymes have been proposed to have a role in the regulation of Na,K-ATPase activity (reviewed in
4 isoform in spermatozoa may be a site of regulation by endogenous ouabain-like compounds. In conclusion, our results provide evidence of a differential cell distribution for the Na,K-ATPase
4 polypeptide in testis cells. This, in addition to the fact that the isoform exhibits unique enzymatic properties, suggests that the
4-subunit may be important in the physiology of the male gonad.
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Acknowledgments |
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Supported by National Institutes of Health grants GM 39746 and DK 45181, and by American Heart Association grant 96012080.
We thank Dr Jeffrey Milbrandt for providing the mice deficient in the Egr-4 transcription factor.
Received for publication February 14, 2000; accepted May 3, 2000.
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