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An anti-NH₂-terminal antibody localizes NBCn1 to heart endothelia and skeletal and vascular smooth muscle cells

Water and Salt Research Center, Institute of Anatomy, University of Aarhus, Aarhus, Denmark

Submitted 1 July 2005 ; accepted in final form 19 August 2005

	ABSTRACT

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The electroneutral sodium bicarbonate cotransporter NBCn1 or NBC3 was originally cloned from rat aorta and from human skeletal muscle. NBCn1 (or NBC3) has been localized to the basolateral membrane of various epithelia, but thus far it has been impossible to detect the protein in these tissues by using anti-COOH-terminal antibodies. Hence an antibody was developed against the NH₂-terminus of NBCn1 and was validated by peptide recognition and immunoblotting on positive control tissues and by binding of an 180-kDa protein in the rat kidney, cerebrum, cerebellum, and duodenum. In addition, an 180-kDa immunoreactive band appeared using samples from the aorta, heart ventricles and atria, mesenteric arteries, lung, spleen, liver, pancreas, and epididymis. Immunohistochemical analysis confirmed the previously described labeling in the kidney, duodenum, and the choroid plexus. The anti-NH₂-terminal antibody localized NBCn1 to the plasma membrane domains of endothelia and smooth muscle cells in small mesenteric and renal arteries, as well as the capillaries of the heart ventricles, spleen, and salivary glands. NBCn1 was also detected in neuromuscular junctions and vasculature in skeletal muscle. Analysis of variable NBCn1 splicing by RT-PCR revealed that an NH₂-terminal sequence, the cassette III, seems absent from cardiovascular NBCn1 and that both cassettes I and III are variable in most epithelia, whereas cassette II is absent from epithelial NBCn1. Thus the development of the NH₂-terminal antibody allowed the localization of NBCn1 protein to major cardiovascular tissues where NBCn1 mRNA was previously detected. The NBCn1 is a likely candidate for mediating the reported electroneutral Na⁺-HCO₃^– cotransport in vascular smooth muscle.

bicarbonate metabolism; acid/base physiology; immunohistochemistry; sodium bicarbonate cotransporter biology

The NBCn1 (or NBC3) has, nevertheless, been suggested to participate in the renal shortcut pathway for NH₄⁺ (13). It was suggested that NBCn1 facilitates influx of NH₄⁺ from the lumen of renal medullary thick ascending limbs by buffering the H⁺ formed along with NH₃ intracellularly after the dissociation of NH₄⁺. NBCn1 is localized to the basolateral plasma membrane in these cells (20) and thus mediates Na⁺ and HCO₃^– uptake from the blood side. The NBCn1 has been localized to the basolateral membrane of other renal tubules as type A intercalated cells of collecting ducts and terminal inner medullary collecting ducts (15, 20). In other epithelia, NBCn1 is also a basolateral protein as in the duodenal mucosa, choroid plexus, and salivary glands (9, 14, 16). Recently, NBCn1 was also found in the rat hippocampal neurons (7). Surprisingly, NBC3 knockout mice revealed no other phenotype than blindness and auditory impairment due to the destruction of neurons in these sensory organs (5). However, there are no reported studies where NBCn1-deficient mice have been challenged by, e.g., the induction of acid/base imbalance, and the implication of NBCn1 in a regulatory response to such conditions is possible.

Originally, NBC3 was cloned from human skeletal muscle (17) and the NBCn1 from rat aorta (6). Nevertheless, it has been impossible to detect the protein in these tissues with the use of the available antibodies directed against the COOH-terminus of NBCn1. Furthermore, the presence of NBCn1 mRNA has been shown in the human heart, rat heart, lung, liver, and spleen by Northern blot analysis or RT-PCR (6, 17). Although the extreme COOH terminus seems to be preserved in all splice variants of NBCn1, none of these tissues has displayed NBCn1 immunoreactivity. Hence it was speculated whether the COOH terminus was somehow masked by either of the at least three variable regions or cassettes of NBCn1. In this study, an anti-NH₂-terminal NBCn1 antibody is used to localize NBCn1 protein in cardiovascular and other tissues that are known to express the NBCn1 encoding mRNA. Furthermore, the initial analysis of NBCn1 splice variation is reported and related to the antibody recognition profile of anti-NH₂-terminal and anti-COOH-terminal antibodies.

	MATERIALS AND METHODS

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Animals. The animal protocols were approved by the Institutional Animal Care and Use Committee, in accordance with the licenses for the care and use of experimental animals issued by the Danish Ministry of Justice. Adult male Wistar rats (300–350 g; from Taconic Europe, Eiby, Denmark) had free access to water and pelleted food (Altromin, Lage, Germany) until use. The rats were anesthetized by isoflurane inhalation before being killed or before perfusion fixation and organ removal.

RT-PCR and sequencing. Total RNA from fresh tissues was extracted with the use of the RNeasy Mini kit (Qiagen, Germantown, MD). After DNase treatment (RQ1 RNase-Free DNase, Promega, Madison, WI), the RNA was reverse transcribed with the use of 2 U/µl reverse transcriptase (Superscript II; Invitrogen, Taastrup, Denmark) in the presence of either poly(T) primers or specific reverse primers for NBC transcripts (gene-specific reverse transcription). PCR (HotStar Taq Master Mix, Qiagen) with 10–20% cDNA and 1 pmol of each primer was performed for 30 cycles: a hot start at 95°C for 15 min, denaturation at 95°C for 30 s, annealing at 56°–60°C (dependent on primer optimum) for 30 s, and elongation at 72°C for 1 min. Negative PCR controls included omission of reverse transcriptase or omission of cDNA. PCR for -actin was performed to validate each batch of template before use. NBCn1 primers were designed to reveal either 5' or 3' variation and are listed in Table 1. PCR products were separated by 2% agarose gel electrophoresis and photographed under ultraviolet illumination. The PCR products in which these were used were previously validated by nucleotide sequencing.

Membrane fractionation and generation of protein samples. Tissues were removed from anesthetized rats that were then decapitated. The tissue samples were homogenized in dissection buffer [0.3 M sucrose, 25 mM imidazole, 1 mM EDTA (pH 7.2), containing 8.5 µM leupeptin and 1 mM phenylmethylsulfonyl fluoride] with the use of an Ultra-Turrax T8 homogenizer (IKA Labortechnik), with two 15-s bursts, and centrifuged at 4,000 g for 15 min at 4°C to remove nuclei, whole cells, and large cellular fragments. The pellet was discarded, and the supernatant was transferred to new tubes. For deglycosylation, 5 µg of the kidney cortex, inner stripe of the outer medulla (ISOM), and inner medulla (IM) samples were incubated overnight with 1 U/10 µl PNGase F (Boehringer-Mannheim). A sample buffer was then added to the samples to obtain a final content of 3% (wt/vol) sodium dodecyl sulfate (SDS), 40.0 mM 1,4-dithiothreitol (DTT), 6% (vol/vol) glycerol, 10 mM Tris (pH 6.8), and bromophenol blue. The samples were heated at 65°C for 5 min and stored at –20°C until use. The total protein content of each sample was determined with the use of the RC DC protein assay (Bio-Rad Laboratories, Herlev, Denmark).

Immunoblotting. Five micrograms of protein from each sample were separated on 7.5% polyacrylamide minigels on a Bio-Rad Mini Protean II system and electrotransferred onto nitrocellulose membranes and then blocked by incubation in 5% skim milk in a phosphate-buffered salt solution [PBS-T, containing 80 mM Na₂HPO₄, 80 mM NaH₂PO₄, 100 mM NaCl, and 0.1% (vol/vol) Tween 20 (pH 7.5)]. The membranes were incubated with primary antibody overnight at 5°C in PBS-T supplemented with 1% BSA and 2 µM NaN₃. After being washed, the membranes were incubated with horseradish peroxidase-conjugated goat anti-rabbit IgG secondary antibody (Dako, Glostrup, Denmark) for 1 h in PBS-T. Excess antibody was removed by extensive washing, and bound antibody was detected by ECL chemiluminescence kit (Amersham, Little Chalfont, UK). Immunoblotting was also performed after the antibody was preincubated with the immunizing peptide for 24 h at 5°C in PBS-T supplemented with 1% BSA and 2 µM NaN₃ to confirm the recognition of the immunogen by the antibody.

Immunohistochemistry. Rat tissues were fixed by perfusion via the abdominal aorta with 4% paraformaldehyde in 0.1 M cacodylate buffer (pH 7.4). The tissues were dehydrated and embedded in paraffin, and 2-µm sections were cut with the use of a rotary microtome (Leica, Heidelberg, Germany). The sections were dewaxed and rehydrated, and endogenous peroxidase was blocked by 0.5% H₂O₂ in absolute methanol. The sections were boiled in 10 mM Tris (pH 9) supplemented with 0.5 mM EGTA and then incubated with 50 mM NH₄Cl and blocked in PBS supplemented with 1% BSA, 0.05% saponin, and 0.2% gelatin. The sections were incubated overnight at 4°C with the primary antibodies diluted in PBS supplemented with 0.1% BSA and 0.3% Triton X-100.

For brightfield microscopy, the sections were incubated with horseradish peroxidase-conjugated goat anti-rabbit IgG (Dako) in PBS with BSA and Triton X-100. The staining was visualized by 0.05% 3,3'-diaminobenzidine tetrahydrochloride dissolved in PBS with 0.1% H₂O₂. Mayer's hematoxylin was used for counterstaining, and the sections were dehydrated in graded alcohol and xylene and mounted in hydrophobic Eukitt mounting medium (O. Kindler, Freiburg, Germany). Microscopy was performed on a Leica DMRE brightfield microscope equipped with a Leica DM300 digital camera.

For fluorescence microscopy, sections were double labeled with primary antibodies against the NH₂ terminus of NBCn1, the AQP-1, or by incubation with -bungarotoxin. The sections were first incubated with the anti-NBCn1 antibody in PBS supplemented with BSA and Triton X-100 with the use of an Alexa 543-conjugated goat anti-rabbit secondary antibody (Molecular Probes, Eugene, OR). The sections were then incubated with a biotinylated anti-AQP-1 with the use of streptavidin FITC (Dako) as the visualizing reagent or -bungarotoxin (Alexa 488 conjugate, Molecular Probes). After being washed, sections were mounted with a coverslip in Glycergel Antifade Medium (Dako) and inspected on a Leica DMRS confocal microscope with an HCX PlApo x64 (1.32 numerical aperture) objective. The immunofluorescence images were merged with differential interference contrast images to reveal the relationship between the tissue structures and the fluorescence labeling.

Immunogold electron microscopy. Tissue blocks prepared from the perfusion-fixed rat hearts [4% paraformaldehyde in 0.1 M cacodylate buffer (pH 7.4)] were cryoprotected with 2.3 M sucrose and rapidly frozen in liquid nitrogen. The samples were freeze-substituted by sequential equilibration over 3 days in methanol containing 0.5% uranyl acetate at temperatures raised gradually from –80° to –70°C, then rinsed in pure methanol for 24 h while the temperature was increased from –70° to –45°C, and infiltrated with Lowicryl HM20 and methanol 1:1, 2:1, and, finally, pure Lowicryl HM20 before ultraviolet polymerization for 2 days at –45°C and 2 days at 0°C. Immunolabeling was performed on ultrathin Lowicryl HM20 sections. Sections were pretreated with a saturated solution of NaOH in absolute ethanol (2–3 s), rinsed, and preincubated for 10 min with 0.1% sodium borohydride and 50 mM glycine in 0.05 M Tris (pH 7.4) containing 0.1% Triton X-100. Sections were rinsed and incubated overnight at 4°C with the NH₂-terminal NBCn1 antibody diluted in 0.05 M Tris (pH 7.4) containing 0.1% Triton X-100 with 0.2% milk. After being rinsed, sections were incubated for 1 h at room temperature with goat anti-rabbit IgG conjugated to 10-nm colloidal gold particles (GAR.EM10; BioCell Research Laboratories, Cardiff, UK). The sections were stained with uranyl acetate and lead citrate before being examined in a Philips Morgagni 268D electron microscope.

	RESULTS

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Validation of the anti-NH₂-terminal NBCn1 antibody. The newly developed antibody was evaluated by means of 1) recognition of the immunizing peptide by the antibody; 2) preabsorption of the antibody with the immunizing peptide before immunoblotting and immunohistochemistry; and 3) finding again the previously described localization. Figure 1A shows that the anti-NH₂-terminal NBCn1 antiserum recognized the immunizing peptide when this was subjected to gel electrophoresis and immunoblotting. Immunoblotting was performed on known positive tissues with the use of either the affinity-purified antibody or the preabsorbed antibody after overnight incubation with the immunizing peptide (Fig. 1B). The expected 180-kDa band is observed in protein samples from the renal cortex/outer medulla, ISOM, and IM, as well as from the heart, cerebrum, cerebellum, and duodenum (Fig. 1B, left). The negative immunodetection after the anti-NBCn1 antibody was preabsorbed is shown in Fig. 1B, right. The two immunoblots were run in parallel. Figure 1C shows the reduction in apparent molecular size of the detected protein resulting from deglycosylation by PNGase treatment. The anti-NH₂-terminal antibody detects the proteins in all three kidney samples (Fig. 1C, left) that are deglycosylated to a similar degree, 40 kDa, as the proteins recognized by the previously characterized anti-COOH-terminal NBCn1 antiserum (Fig. 1C, right). The results indicate that the anti-NH₂-terminal antibody recognizes the same N-glycosylated protein as the anti-COOH-terminal NBCn1 antiserum.

View larger version (41K): [in this window] [in a new window]   Fig. 1. Immunoblot validation of anti-NH2-terminal NBCn1 antibody. A: peptide recognition by anti-NH2-terminal NBCn1 antibody. After SDS-PAGE, immunizing peptide was electrotransferred onto nitrocellulose and incubated with anti-NH2-terminal NBCn1 antiserum and visualized by chemiluminescence with use of horseradish peroxidase-conjugated secondary antibody. B: preabsorption test of anti-NH2-terminal NBCn1 antibody. Selected ranges of known positive tissues were subjected to immunoblotting with affinity-purified anti-NH2-terminal (Nt) NBCn1 antibody (left) or same antibody after overnight incubation with immunizing peptide (right). Lanes represent renal cortex and outer stripe of outer medulla (Ctx), renal inner stripe of outer medulla (ISOM), and renal inner medulla (IM), sample buffer (SB), heart, cerebrum (Cbr), cerebellum (Cbll), and duodenum (Duod). C: effect of deglycosylation on protein migration. Samples from rat kidney were treated enzymatically with PNGase F (dg) and immunoblotted with use of anti-NH2-terminal NBCn1 (left) on samples from rat kidney. Anti-COOH-terminal (Ct) NBCn1 antiserum was applied on ISOM samples (right).

View larger version (124K): [in this window] [in a new window]   Fig. 2. Immunohistochemical localization of NBCn1 in known positive tissues. Anti-NH2-terminal NBCn1 antibody was applied to semithin sections of rat kidney, duodenum, and brain for immunohistochemical verification of antibody sensitivity. A: immunolabeling in transition between ISOM and IM. Dashed line marks transition and arrows mark basolateral plasma membrane domain of medullary thick ascending limbs (mTAL) of Henle's loop and a subset of collecting duct cells in ISOM (OMCD) and initial inner medulla (IMCD1). B: immunostaining of terminal inner renal medulla. Arrows mark collecting duct cells (IMCD3). C: duodenal mucosa subjected to anti-NBCn1 immunolabeling. Arrows show basolateral plasma membrane domain of villus enterocytes. Lp, lamina propria. D: immunolabeling in rat brain. Basolateral plasma membrane domain of choroid plexus epithelium is marked by arrows. Bl, blood side of epithelium; Ar, arteriole. Scale bars = 50 µm. Insets show result of preabsorbing the antibody with immunizing peptide.

View larger version (42K): [in this window] [in a new window]   Fig. 3. Comparison of protein detection by anti-NH2-terminal and anti-COOH-terminal NBCn1 antibodies. A: immunoblot performed with use of anti-NH2-terminal NBCn1 antibody on various rat tissue samples. Mesenteric a, mesenteric arteries; cortex, renal cortex and outer stripe of outer renal medulla; Submandib gl, submandibular gland; Subling gl, sublingual gland. B: immunoblot performed in parallel with immunoblot in A, with application of the previously described anti-COOH-terminal NBCn1 antiserum. C: immunoblot performed with use of anti-NH2-terminal NBCn1 antibody on protein samples from rat ISOM and rat skeletal muscle (Sk Musc, from entire quadriceps femoris muscle).

View larger version (111K): [in this window] [in a new window]   Fig. 4. Immunohistochemical localization of NBCn1 in rat blood vessels. Blood vessels from semithin sections of various tissues were stained with anti-NH2-terminal antibody. A: immunostaining of the aorta. Arrows mark endothelium (Endo) and an arteriole (A) in tunica adventitia. B: immunolabeling of a mesenteric artery. Arrows mark endothelium and smooth muscle cells in tunica media. C: immunoreactivity of a renal cortical small artery. Arrows mark endothelium and smooth muscle cells in tunica media. D: hepatic NBCn1 staining. Portal triad of portal vein, hepatic artery (Ar), and interlobular bile duct (Bi) are shown. Scale bars = 50 µm.

View larger version (112K): [in this window] [in a new window]   Fig. 5. Immunohistochemical localization of NBCn1 in rat heart and skeletal muscle. A: immunostaining of heart atrium (Atr). C, capillaries. B: immunolabeling of ventricle wall. C, capillaries. C: double-staining immunofluorescence detection of NBCn1 (red) and endothelial water channel (green). Colocalization is coded yellow, and fluorescence signals are superimposed on a differential interference contrast image. CM, cardiomyocytes; C, capillaries. D: immunogold electron micrograph of a capillary from rat atria. IN, interstitial tissue; En, endothelium; Nu, nuclei. Arrows indicate gold particles. E: immunolabeling of skeletal muscle. M, myocytes; C, capillaries. Arrows indicate neuromuscular junctions. F: double labeling of skeletal muscle for NBCn1 (red) and -bungarotoxin (green). Colocalization is coded yellow, and fluorescence signals are superimposed on a differential interference contrast image. M, myocytes; C, capillaries. Arrows indicate neuromuscular junctions. Scale bars = 50 µm in A and B; 25 µm in C and E; 10 µm in F; 500 nm in D. Insets in A and B show result of preabsorbing the antibody with immunizing peptide.

RT-PCR analysis of NBCn1 splice variation. RT-PCR was performed on selected tissues to confirm the presence of NBCn1 RNA in the different tissues and to investigate whether there was a connection between the presence of the cassettes I, II, and III and the ability of the anti-NH₂-terminal and anti-COOH-terminal NBCn1 antibody to recognize the protein. Figure 6A shows the products after RT-PCR with the use of a primer pair to amplify the cassettes I and II of NBCn1. The higher-molecular-weight band indicates the presence of cassette I, and a lower band indicates its absence. Both the presence and absence of cassette I were found in the ISOM and IM of the kidney, in cerebrum, cerebellum, pylorus, duodenum, ileum, colon, the submandibular, sublingual, and parotid glands, trachea, spleen, and epididymis. No bands were detected in the liver and heart under these reaction conditions, nor was the cassette II detected in any tissues because the reaction theoretically should yield a product size of 766 bp. Figure 6B shows similar analysis of the presence of cassette III. Although inclusion of cassette III seemed to dominate in most tissues, mRNA excluding cassette III was found in the ISOM and IM of the kidney, cerebellum, duodenum, ileum, liver, trachea, spleen, and epididymis. In the rat heart, the product indicating the absence of cassette III was dominating. Thus the expression of both cassettes of NBCn1 seems to vary at the mRNA level within a variety of epithelial tissues.

View larger version (21K): [in this window] [in a new window]   Fig. 6. PCR analysis of tissue expression pattern of various NBCn1 splice variants. Primers were designed to amplify a sequence spanning both cassettes I and II of NBCn1 (A) or cassette III (B) in various rat tissues. Expected product sizes were 397 bp in presence of cassette I and 358 bp in its absence. Addition of cassette II would yield an additional 369 bp. Expected products for cassette III fragment were 334 bp in its presence and 223 bp in its absence. Cbl, cerebellum; Pyl, pylorus; Duo, duodenum; Ile, ileum; Col, colon; Panc, pancreas; Liv, liver; Atr, heart atrium; Ventr, heart ventricle; Gl SM, submandibular gland; Gl SL, sublingual gland; Gl Par, parotid gland; Trach, trachea; Lun, lung; Spl, spleen; Epid, epididymis.

	DISCUSSION

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

Immunoblotting with the use of the anti-NH₂-terminal NBCn1 antibody shows three apparently distinct bands: a fuzzy 180-kDa band, a sharp 180-kDa band, and an 140-kDa band. It seems as though the fuzzy band is found in tissues where immunohistochemistry reveals epithelial staining and the sharp band is found in tissues where the endothelium is primarily labeled. Preparations of isolated renal medullary thick ascending limbs or duodenal enterocytes yield only the 180-kDa broad band (not shown). The variations in band appearance in the different tissues and sometimes within a single tissue may possibly be accounted for by differences in glycosylation and phosphorylation of the protein or by variable splicing.

One reason the anti-NH₂-terminal antibody recognizes NBCn1 in more tissues by immunoblotting may be that there is a structural hindrance for recognition by the anti-COOH-terminal or anti-hNBC3 antibodies. It has been speculated that the COOH-terminus is bound to cytoskeletal or other proteins in a way that masks the epitope for the anti-COOH-terminal and anti-hNBC3 antibodies. This is unlikely because the proteins are detached and denatured during immunoblotting. Thus a simpler explanation would be that the anti-NH₂-terminal antibody reveals NBCn1 immunoreactivity with a better signal-to-noise relationship than the previous antibodies. The difference in histochemical labeling patterns may, however, rely on splice variation, by which one or more of the variable sequences could mask or otherwise hinder recognition of the epitope.

Three variable regions have been described in the NBCn1. The cassette I consists of 14 amino acids in the long intracellular NH₂-terminus and was formerly called the A-cassette; cassette II is the following 123 amino acids; and cassette III, formerly the B-cassette, consists of 36 amino acids in the COOH-terminus (7). It appears that both cassettes I and III are variable in epithelial NBCn1, whereas cassette II seems absent from epithelial NBCn1. Interestingly, the cassette III is absent from the heart, showing a substantial lower band. This feature seems to coincide with the lack of recognition by the anti-COOH-terminal NBCn1 antibodies that may only recognize the "epithelial NBCn1." It remains to be clarified how many of these transcripts are converted into biologically significant amounts of NBCn1 protein and whether the apparent difference in epithelial and nonepithelial NBCn1 can be confirmed at the protein level.

Table 2 provides a summary of the expression profile for NBCn1 found in a range of tissues by RT-PCR, immunoblotting, and immunohistochemistry. Overall, there is good correlation among the results obtained with the three techniques. The expression of NBCn1 in the cardiovascular structures was found by all three methods, as was the staining in the brain and epididymis. PCR analysis of NBCn1 expression was not performed for the aorta and other arteries in the present study but was previously shown by the cloning from an aorta library (6). The novel staining of the aorta is interesting because NBCn1 was not detected in this tissue by using the previously applied antibodies. The labeling of endothelia and vasa vasorum appears credible, but the staining of smooth myocytes is less compelling. The staining in these cells seems to be cytosolic, which is a highly unlikely position for a protein that does not undergo acute regulated vesicular trafficking. Moreover, NBCn1 is indeed observed in close proximity to the plasma membrane domain of small-artery myocytes in both the kidney and the mesentery. This is interesting because all prior attempts to detect NBCn1 protein in vascular smooth muscle have failed. Na⁺-dependent HCO₃^– transport has been described in vascular smooth muscle from mesenteric arteries (1). This transport process has been shown to be DIDS sensitive and electroneutral. Interestingly, the vascular NBCn1 is apparently inhibited by this compound, whereas the epithelial form seems relatively DIDS insensitive. Evidence for endothelial Na⁺-dependent HCO₃^– transport is sparse, but such transport has been observed in primary cultures of brain endothelia (C. Taylor, M. Barrand, and S. Hladky, Department of Pharmacology, Cambridge University, UK, personal communication). It remains to be clarified whether this transport is indeed mediated by NBCn1.

A band is detected by immunoblotting in all the tissues of the GI tract from corpus and fundus of the stomach to colon as well as in the liver and pancreas. Whereas NBCn1 was readily detected in the small intestine including the duodenum by immunohistochemistry, the protein was not detected in the pylorus and colon by this method. This could rely on masking of both the COOH-terminal and NH₂-terminal epitopes selectively in these tissues, although this remains an uncorroborated explanation for the lack of labeling. In the salivary gland, there also may be some discrepancies in the results. PCR and immunohistochemistry shows the presence of NBCn1 in all three salivary glands. However, the immunoblotting shows absence of labeling in the submandibular and sublingual glands. The reason for this inconsistency might again rely on relatively low NBCn1 abundance in the glands. NBCn1 staining was primarily found in vascular and ductal structures, which comprise a small fraction of the tissue, and these structures would not be well represented in the loaded proteins in immunoblotting. Nevertheless, previous studies have detected NBCn1 in the rat parotid and submandibular glands (9). In that study, the presence of NBCn1 RNA in these tissues was confirmed by immunoblotting, but immunohistochemical analysis only showed weak labeling of submandibular gland and no labeling of parotid gland.

In conclusion, an anti-NH₂-terminal NBCn1 antibody localized the electroneutral Na⁺-HCO₃^– cotransporter for the first time to cardiovascular tissue and to skeletal muscle. NBCn1 was expressed in the endothelia of large arteries, in small arteries, in capillaries of many epithelial tissues, in heart atria and ventricles, and in skeletal muscle. NBCn1 was also found in vascular smooth muscle of small arteries and in the neuromuscular junction of skeletal muscle. The findings call for further investigations into the functional role of NBCn1 in endothelia and muscle.

	GRANTS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
H. H. Damkier was supported by Aarhus University Research Foundation (Aarhus Universitets Forsknings Fond). Support was also granted from The Novo Nordic Foundation and The Danish Medical Research Council (Statens Sundhedsvidenskabelige Forskningsråd). The Water and Salt Research Center at the University of Aarhus was established and supported by the Danish National Research Foundation (Danmarks Grundforskningsfond).

	ACKNOWLEDGMENTS

 
We thank Prof. Christian Aalkjaer and Assoc. Prof. Helle A. Praetorius, Institute of Physiology, University of Aarhus, for valuable discussions and comments to the manuscript. Also, Inger Merete S. Paulsen, Zhila Nikrozi, Mette F. Vistisen, and Helle Hoyer are thanked for expert technical assistance and training.

	FOOTNOTES

 

Address for reprint requests and other correspondence: J. Praetorius, Water and Salt Research Center, Institute of Anatomy, Univ. of Aarhus, Wilhelm Meyers Allé, Bldg. 234, 8000 Aarhus C, Denmark (e-mail: jp{at}ana.au.dk)

The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

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