Functional Domains and Expression of Truncated Atrial Natriuretic Peptide Receptor-A: The Carboxyl-Terminal Regions Direct the Receptor Internalization and Sequestration in COS-7 Cells

Experimental Procedures

Materials.

ANP (rat-28) was purchased from the Peninsula Laboratories, Inc. (Belmont, CA). Na-¹²⁵I (100 mCi/ml; carrier free) andl-[³⁵S]methionine (1000 Ci/mmol) were obtained from Amersham Pharmacia Biotech Inc. (Piscataway, NJ). Erase-a-base kit was obtained from Promega (Madison, WI). Restriction enzymes were purchased from Stratagene (La Jolla, CA). The mammalian expression vector p^cDNA3 was obtained from InVitrogen (San Diego, CA). cGMP radioimmunoassay kit was purchased from the Biomedical Technologies, Inc. (Stoughton, MA). Succinimido-4-azidobenzoate was obtained from Pierce (Rockford, IL). Tissue culture supplies were received from Life Technologies (Grand Island, NY). All other chemicals were molecular biology reagent grade.

Plasmid Construction.

Full-length murine Npra cDNA (Pandey and Singh, 1990) was excised from Bluescript vector by digesting withNotI and was then subcloned into a site of p^GEM5zf(+) vector previously digested byNotI. The ligated inserts in opposite orientation (3′-5′ direction) were used for deletion mutagenesis. Plasmid vector p^GEM5zf(+) containing the cDNA insert was linearized by SphI restriction enzyme. An adaptor containing two additional restriction sites (NotI and SnBI) was ligated between AtaII and SphI sites in multiple cloning regions of p^GEM5zf(+) vector. The primers (5′-c t a c g t a g c g g c c a c a c a t g-3′ and 3′-g t a c g a t g c a t c g c c g g c g t-5′) with 1/2 SphI site were synthesized and annealed to each other to prepare the cassette. Plasmid p^GEM5zf(+) was digested with restriction enzyme SphI and the DNA cassette was ligated at the SphI site. After ligation of the cassette to the plasmid, the left SphI site was regenerated; however, the right SphI site was not regenerated because of a single-base mismatch to the original site. Plasmid p^GEM5zf(+)was linearized by double digestion using SphI andSpeI restriction endonucleases. Restriction enzymesSphI and SpeI generated exonuclease III resistant sites at the 3′ and 5′ ends, respectively. A complete series of exonuclease III digestion and S1 nuclease treatment was performed using a Promega Erase-a-base kit, according to the method ofHenikoff (1984). The DNA ends were filled using Klenow polymerase and ligated according to the manufacturer's protocols. The plasmids were prepared, and the sizes of deleted cDNAs were confirmed by nucleotide sequencing. All deleted Npra cDNAs were excised from p^GEM5zf(+) vector by digesting with restriction enzyme NotI and were then subcloned into a site of the mammalian expression vector p^cDNA3 that had been previously digested by NotI. The vector p^cDNA3 was reconstructed using an adaptor containing the termination codon in all reading frames at theXhoI site. The expression vector p^cDNA3 is designed to function under the control of cytomegalovirus immediate early promoter and contains the simian virus-40 origin of replication to increase the transient expression of encoded protein in transfected cells. Restriction mapping and DNA sequencing to verify the correct reading-frame of ligated cDNA inserts [according to the method of Tabor and Richardson (1987)] identified the plasmids of interest that had inserts in correct orientation.

Production of Rabbit Polyclonal Antibodies.

The peptide Lys-Cys-Gly-Phe-Asp-Asn-Glu-Asp-Pro-Ala-Cys-Asn-Gln-Asp-His-Phe-Ser-Thr, corresponding to 18 amino-terminal residues (450–467) in the extracellular domain adjacent to the transmembrane domain of Npra, was conjugated to keyhole limpet hemocyanin. The keyhole limpet hemocyanin-peptide conjugate was injected i.p. in the presence of complete Freund's adjuvant into rabbit 809 and 810 (Immuno-Dynamics, Inc., La Jolla, CA). The rabbits were boosted four times with peptide in Freund's incomplete adjuvant. The antiserum was purified using the Thiopropyl-Sepharose 6B matrix (Pharmacia, Piscataway, NJ).

Transfection and Receptor Binding Assay.

COS-7 cells were grown in Dulbecco's modified Eagle's medium (DMEM) supplemented with 10% fetal bovine serum (FBS) at 37° in an atmosphere of 5% CO₂ and 95% O₂. Cells were transfected with plasmids containing either full-length or deleted Npra cDNAs. Transfection was performed by electroporation using 20 μg of plasmid DNA at 220 V with a capacitance setting of 960 μF using a gene Pulser (BioRad, Richmond, CA). After electroporation, cells were seeded into 60-mm² culture dishes. The medium was changed after 24 h and functional studies were performed 48 h after transfection. Rat ANP-28 was iodinated with Na-¹²⁵I (100 mCi/ml; carrier free) by the Chloramine-T method as described previously (Pandey et al., 1986,1988). ANP-binding was measured essentially as described elsewhere (Pandey, 1992, 1993). Briefly, cells were washed three times with assay medium (DMEM containing 0.1% bovine serum albumin) and incubated at 4°C in 2 ml of fresh assay medium, containing 1 nM¹²⁵I-ANP in the presence or absence of 100 nM unlabeled ANP. After the binding was completed, the medium was removed and cells were washed four times with ice-cold assay medium and dissolved in 0.5N NaOH. ¹²⁵I-ANP radioactivity was counted.

Photoaffinity Labeling, SDS-Polyacrylamide Gel Electrophoresis (PAGE), and Autoradiography.

The photoaffinity ligand azidobenzoyl-¹²⁵I-ANP (AZB-¹²⁵I-ANP) was prepared as described previously (Pandey et al., 1986, 1988). Forty-eight hours after transfection, cells were washed with assay medium and then incubated at 4°C in fresh medium containing AZB-¹²⁵I-ANP in the presence or absence of unmodified ANP for 10 min in dark as described elsewhere (Pandey, 1992, 1993). After binding, cells were washed three times with ice-cold assay medium and photolyzed in fresh medium. Cells were then rewashed four times with assay medium and lysed in a solution containing 0.5% SDS, 1% Triton X-100, 1 mM phenylmethylsulfonyl fluoride, 2 mM N-ethylmalemide, 10 μg/ml leupeptin, and 10 μg/ml aprotinin. The aliquots of the cell lysates were boiled for 5 min with equal volumes of sample buffer and analyzed by SDS-PAGE using 7.5% gels under reduced conditions according to the method of Laemmli (1970). Electrophoresis was carried out at a constant current of 25 mA until the bromphenol blue front reached the bottom of the gel. Proteins in the gel were stained with Coomassie Brilliant blue R-250. After destaining, gels were dried and autoradiographed at −70°C using Kodak X-Omat film and Cronex Lightning Plus (DuPont, Boston, MA) intensifying screen. The proteins used for standard molecular weight (i.e., relative molecular mass) calibration were as follows: myosin (M _r205,000), β-galactosidase (M _r 116,000), phosphorylase b (M _r 97,000), bovine serum albumin (M _r 67,000), ovalbumin (M _r 45,000) and carbonic anhydrase (M _r 29,000).

cGMP Assay.

Forty-eight hours after transfection, cells were treated with ANP at 37°C for 10 min in the presence of 0.2 mM 3-isobutyl-1-methylxanthine. Cells were washed three times with PBS and scraped in 0.5N HCl. Cell suspensions were placed in a boiling-water bath for 3 min and centrifuged at 1500g for 15 min at 4°C. Supernatants were collected and lyophilized. Samples were reconstituted with acetate buffer and recentrifuged. In supernatants, the cGMP contents were determined by radioimmunoassay kit as described previously (Khurana and Pandey, 1995).

Metabolic Labeling of transfected COS-7 Cells with [³⁵S] Methionine.

COS-7 cells were transfected with wild-type and carboxyl-terminal deleted Npra cDNAs and plated in 60-mm² dishes containing DMEM supplemented with 10% FBS. Twenty-four hours after transfection, a pulse-chase experiment was performed by washing the attached cells twice with Hanks' balanced salt solution (HBSS) and incubating at 37°C with 2 ml of methionine-free DMEM supplemented with 1 μM unlabeled methionine, 10% FBS, and 0.15 mCi/mll-[³⁵S]methionine. After 30 min, the pulse medium was removed. The cells were washed once with HBSS and 3 ml of chase medium consisting of normal DMEM and 10% FBS and incubated in fresh medium at 37°C for 18 h. After incubation, the chase medium was removed, and the cells were washed with HBSS and scraped in solubilizing buffer (20 mM HEPES, pH 7.4, 150 mM NaCl, 10% glycerol, 1% Triton X-100, 5 mM EDTA, 1 mM phenylmethylsulfonyl fluoride, 20 μg/ml aprotinin, and 20 μg/ml leupeptin). Cell lysate was stirred for 30 min at 4°C and the mixture was centrifuged for 5 min at 1,000g to remove the insoluble material and then recentrifuged at 100,000g for 60 min to obtain the clear supernatant, which contained the solubilized receptors.

Immunoprecipitation.

For immunoprecipitations, equal amounts of proteins (100 μg) obtained from cells expressing the wild-type or carboxyl-terminal deleted receptors were incubated with 1:400 dilution of Npra antiserum at 4°C for 4 h. The immunocomplex was precipitated with protein-A agarose, and nonspecific proteins were removed by washing the precipitated material four times with radioimmunoprecipitation assay buffer containing 20 mM Tris · HCl, pH 7.8, 150 mM NaCl, 1% sodium deoxycholate, 1% Triton X-100, and 0.2% SDS, as described previously (Pandey, 1994). The contents were dissolved in Laemli's sample buffer, boiled for 5 min, and the immunoprecipitated proteins were analyzed by SDS-PAGE and fluorography.

Receptor Internalization and Sequestration.

Transfected COS-7 cells were plated in 60-mm² dishes and cultured at 37°C in an atmosphere of 5% CO₂and 95% O_2. Forty-eight hours after transfection, cells were washed three times with assay medium and incubated in the presence of ¹²⁵I-ANP at 4°C for increasing time periods. The internalization experiments were performed as described previously (Pandey, 1993). The unbound¹²⁵I-ANP was removed by extensive washing with cold assay medium and total cell-associated radioactivity was determined by dissolving the cells in 0.5N NaOH, which accounted for the initial zero time control value of 100%. After completion of the binding, cells were quickly warmed to 37°C to allow the internalization of ligand-receptor complexes. At the indicated times, culture dishes were removed from 37°C and placed on ice, and medium was collected to determine the release of both degraded and intact ligands. The cell surface-associated radioactivity was removed by washing the cells with ice-cold acidic buffer (50 mM glycine/100 mM NaCl, pH 3.8) at 4°C. After acid wash, the internalized¹²⁵I-ANP radioactivity was measured by dissolving the cells in 0.5N NaOH. To determine the rate of lysosomal degradation of ligand-receptor complexes, the cells expressing the wild-type and truncated receptors were pretreated with the lysosomotropic agent chloroquine (200 μM) at 37°C for 45 min and then allowed to bind¹²⁵I-ANP at 4°C for 1 h. The amount of intact and degraded products in the medium was determined by precipitation with 10% trichloroacetic acid (TCA) containing 200 μl of bovine serum albumin (5%) as carrier. The supernatants contained the degraded products and precipitates of TCA retained the intact¹²⁵I-ANP.

Results

To characterize the functional properties of the intracellular domains of Npra, a full-length (1057 aa residues) cDNA insert was sequentially deleted from the 3′ end extending to near the transmembrane domain of the receptor. We generated a series of functional truncated Npra inserts by sequentially deleting the aa residues at the carboxyl-terminal end of the receptor (e.g., −12 aa, −120 aa, −141 aa, −155 aa, −170 aa, −422 aa, or −569 aa). The stop codon was provided at the carboxyl-terminal end of each insert after the aa residue; 1045, 937, 916, 902, 887, 637, or 488, respectively, as stated under Experimental Procedures. The resultant truncated mutant receptors were designated as Δ1045-Npra, Δ937-Npra, Δ916-Npra, Δ902-Npra, Δ887-Npra, Δ635-Npra, and Δ488-Npra, respectively, and are represented diagrammatically in Fig.1. Both the wild-type and mutant cDNAs were transiently expressed into COS-7 cells, and 48 h after transfection, functional studies were carried out. Deletion of 12-aa residues (Δ1045-Npra) at the carboxyl-terminal end of the receptor did not affect the ligand binding (Fig.2). However, the removal of most of the guanylyl cyclase catalytic domain, up to 120 to 170 aa of receptor (Δ937-Npra, Δ916-Npra, Δ902-Npra, and Δ887-Npra), exhibited approximately 20% reduction in ANP-binding compared with wild-type or 12-aa-deleted (Δ1045-Npra) receptors. The deletion of 422 aa residues (Δ635-Npra), including the guanylyl cyclase catalytic domain and the KHD, resulted in almost 50% reduction in ligand-binding capacity of the receptor. Approximately, 85 to 90% of¹²⁵I-ANP binding was reduced in COS-7 cells expressing the −569 aa truncated (Δ488-Npra) receptor (Fig. 2).

To determine the binding of AZB-¹²⁵I-ANP to wild-type or truncated mutant receptors, we performed photoaffinity labeling of expressed receptors in COS-7 cells. Consistent with¹²⁵I-ANP binding assay, photoaffinity labeling of ligand-receptor complexes indicated a reduced binding of AZB-¹²⁵I-ANP to Δ635-Npra compared with the wild-type receptor protein (Fig. 3). The AZB-¹²⁵I-ANP-labeled recombinant wild-type Npra, and the truncated (Δ635-Npra) mutant receptors were separated by SDS-PAGE as discrete protein bands with the expected molecular masses of 135 kDa and 81 kDa, respectively. The expression of wild-type Npra in COS-7 cells resulted in an ANP-dependent accumulation of intracellular cGMP by more than 35-fold. The deletion of 12 aa residues at the carboxyl-terminal end (Δ1045-Npra) did not show any discernible effect on cGMP production in response to ANP stimulation (Fig. 4). Nevertheless, deletion of 120 aa (Δ937-Npra) in the guanylyl cyclase catalytic domain of Npra resulted in a 40 to 45% reduction in the intracellular accumulation of cGMP. Further deletion of 141 aa residues (Δ916-Npra) in the guanylyl cyclase catalytic domain blocked more than 95% of ANP-dependent intracellular accumulation of cGMP. To assess the specificity of cGMP production by wild-type or carboxyl-terminal-deleted cDNA constructs, we used the Npra antagonist A-71915. The receptor antagonist A-71915 blocked the generation of cGMP in response to ANP-treatments in COS-7 cells expressing both the wild-type and mutant receptors (Fig. 4). The results of immunoprecipitation studies indicated that wild-type and carboxyl-terminal-deleted receptors are expressed on the cell surface without a significant decrease in the protein contents of mutant receptors (Fig. 5). The wild-type and several mutant receptors showed almost equivalent levels of protein expression in immunoprecipitates, except that the expression of Δ488-Npra was significantly reduced compared with all other truncated mutant receptors.

We examined whether guanylyl cyclase catalytic and/or protein KHDs are required for internalization and intracellular sequestration of Npra. For this purpose, we determined the cell-surface associated, internalized and released ¹²⁵I-ANP radioactivity in COS-7 cells expressing the wild-type or sequentially truncated cDNA inserts. We distinguished between the surface-associated, internalized and released ¹²⁵I-ANP radioactivity by acid wash procedure as described under Experimental Procedures. Forty-eight hours after transfection, cells in 60-mm² culture dishes were allowed to bind ¹²⁵I-ANP at 4°C for 1 h. After this, unbound ¹²⁵I-ANP was removed by washing the cells with assay medium, and cells in culture dishes were then incubated in fresh medium at 37°C to allow the internalization of ligand-receptor complexes inside the cell. At the indicated time periods, culture dishes in replicates were removed from 37°C, and media was collected. Cells were washed once with HBSS and then treated with glycine acidic buffer (pH 3.8) at 4°C to release the cell-surface associated¹²⁵I-ANP (Fig.6a). At the initial internalization period (zero time), approximately 85% of the cell-surface bound ¹²⁵I-ANP radioactivity was released by acid-treatment of cells expressing the wild-type or 12 aa deleted (Δ1045-Npra) receptors. However, a continued reduction in cell-surface binding was observed with all other carboxyl-terminal-deleted receptors. Approximately 60 to 65% of¹²⁵I-ANP binding was observed in cells expressing the Δ937-Npra or Δ887-Npra, and only 40% of¹²⁵I-ANP binding was detected in cells that expressed the Δ635-Npra compared with wild-type receptors (Fig. 6a). After the acid wash, the cells in culture dishes were dissolved in 0.5 N NaOH to quantify the internalized ¹²⁵I-ANP. We observed that after 5 min incubation at 37°C, approximately 35 to 40% ¹²⁵I-ANP remained inside the cells that expressed wild-type receptors, and only 20 to 25%¹²⁵I-ANP was localized in cells expressing the Δ937-Npra or Δ887-Npra mutant receptors (Fig. 6b). However, an almost negligible amount of ¹²⁵I-ANP was detected inside the cells that expressed either Δ635-Npra or vector DNA. The data presented in Fig. 6c show that after a 30-min incubation at 37°C, cells expressing the wild-type Npra or Δ1045-Npra released almost 80% internalized ¹²⁵I-ANP. The release of¹²⁵I-ANP was reduced to 60% in cells that expressed Δ937-Npra or Δ887-Npra; however, only 10 to 15%¹²⁵I-ANP was released from the cells expressing the Δ635-Npra.

The COS-7 cells expressing the wild-type or mutant receptors were pretreated with the lysosomotropic agent chloroquine at 37°C for 30 min. The release of ¹²⁵I-ANP in culture media of cells, expressing the wild-type receptors, was blocked by chloroquine during a 15-min incubation (Fig. 7a). However, after an extended period of incubation (30–60 min), the effect of chloroquine diminished, and a large amount of internalized¹²⁵I-ANP radioactivity was released into culture media (Fig. 7b). We observed that with increasing deletions of aa residues at the carboxyl-terminal end of receptor, a large proportion of ligand-receptor complexes did not internalize and remained on the cell-surface (Fig. 7, a and b). The quantitative assessment of the intact and degraded ligand was determined by measuring the solubility of ¹²⁵I-ANP products in 10% TCA. The TCA precipitates (intact ligand) and supernatants (degraded ligand) were separated by centrifugation. The released¹²⁵I-ANP consisted of higher amounts of degraded products and a lesser amount of intact ligand in culture media of the cells expressing either wild-type or carboxyl-terminal truncated mutant receptors (Fig. 8, a and b).

Discussion

To investigate the structure-function relationship of the KHD and guanylyl cyclase catalytic domain of Npra, we studied whether the sequential deletion of aa from the carboxyl-terminal end of Npra would render the overall function undetected. We made nested sets of sequential deletions throughout the intracellular region covering both the guanylyl cyclase catalytic and protein KHDs of Npra to determine the specific sequence regions within these domains that should be important for modulation of the functional activity of this receptor protein. The data show that deletion of carboxyl-terminal regions of Npra affects the ligand-binding activities, cGMP production, and internalization and sequestration of ligand-receptor complexes in COS-7 cells expressing the mutant receptors. The present studies have relied on the loss of function of deletion mutations to identify the regions within the KHD and guanylyl cyclase catalytic domain of Npra for postbinding events and receptor function. The guanylyl cyclase/natriuretic peptide receptors (Npra, Nprb) are unique in nature because they contain distinct ligand-binding, transmembrane, protein kinase-like homology and guanylyl cyclase catalytic domains (Garbers, 1992). The natriuretic peptide receptor-C (Nprc) which also contains a single transmembrane domain with a short (37 aa residues) cytoplasmic tail, is considered to clear ANP from the circulation; hence, it is named the clearance receptor (Maack, 1992). However, recent studies with Nprc-gene-knockout mice have shown that Nprc might also be involved in certain critical biological functions displayed by ANP (Matsukawa et al., 1999). All three natriuretic peptide receptors have several common characteristics in the extracellular ligand-binding domains (Itakura et al., 1994, 1997; Takashima et al., 1995).

Although considerable efforts have been made to define the structure-function relationship of Npra, sufficient studies have not been carried out using the sequential deletion strategy of the carboxyl-terminal end to define the high-order structure characteristics of this receptor protein. In the present studies, we have identified regions in KHD and guanylyl cyclase catalytic domain of Npra by deletion mutagenesis that seem to play important roles in ligand-binding, cGMP production, and metabolic turn-over of this receptor protein. In COS-7 cells expressing the recombinant Npra,¹²⁵I-ANP binds to cell-surface receptors, enters through the process of receptor-mediated endocytosis, and are rapidly released into culture media, which is a process similar to that observed with endogenous native receptors (Pandey, 1993). Our results show that deletion of a large part of guanylyl cyclase domain did not seem to have a major effect on the affinity of ANP-binding. However, cells expressing Δ635-Npra or Δ488-Npra mutant receptors showed approximately 50% and 80% reduction in ¹²⁵I-ANP binding, respectively, compared with the cells expressing full-length wild-type receptor protein. The immunoprecipitation studies indicated that wild-type and carboxyl-terminal-deleted receptors are expressed on the cell surface without a significant decrease in protein contents of mutant receptors, except that the expression of Δ488-Npra was significantly reduced. These results establish that the reduction in binding affinity of Δ937-Npra, Δ916-Npra, Δ887-Npra, or Δ635-Npra is primarily caused by a loss of specific sequence regions in the intracellular domain of Npra. However, the expression of Δ488-Npra protein was slightly reduced; therefore, it can be assumed that the reduction in ligand-binding affinity of Δ488-Npra might be contributed, because of a loss of specific sequence region of KHD in the amino terminus of Npra, and partly because of its reduced expression on the cell surface.

Deletion of 12 aa residues (Δ1045-Npra) at the carboxyl-terminal end of receptor did not seem to affect ligand binding, cGMP stimulation, or internalization of Npra. However, further deletions at the carboxyl-terminal end of Npra dramatically diminished the extent of ligand binding, cGMP production, and internalization of ligand-receptor complexes in COS-7 cells expressing the mutant receptors. Previous studies have suggested that endogenous native ANP receptors Nprc (Nussenzveig et al., 1990; Pandey, 1992; Rathinavelu and Isom, 1991,1993) as well as Npra (Pandey, 1993) are rapidly internalized in intact cells. Nevertheless, the exact mechanism of endocytosis of these receptors remains to be established. Our deletion mutagenesis studies, aimed at identifying the specific functional regions, revealed that the sites within the intracellular KHD and guanylyl cyclase catalytic domain of Npra seem to play an important role in endocytosis and intracellular sequestration of this receptor protein. The ligand-binding kinetics of wild-type recombinant Npra showed that the ligand-receptor complexes were rapidly internalized and both the intact and degraded ligands were released into culture media in a manner similar to those of native endogenous receptors (Pandey, 1993). Similarly, it has been shown that endocytotic rates of transfected recombinant Nprc into Chinese hamster ovary cells were comparable with that described for native Nprc (Cohen et al., 1996). These authors suggested that the internalization signal for Nprc is located in the cytoplasmic domain and complete deletion of this domain virtually disrupted the internalization of the receptor, reducing the net endocytotic rate by approximately 10-fold compared with the full-length wild-type receptors.

Data presented herein demonstrate a differential pattern of receptor-mediated lysosomal hydrolysis of¹²⁵I-ANP in COS-7 cells expressing the recombinant wild-type Npra and the carboxyl-terminal truncated forms of mutant receptors. Our results suggest that truncation of Npra at the carboxyl-terminal end significantly reduced the hydrolysis of ligand-receptor complexes compared with the wild-type receptor. For example, the expression of Δ937-Npra and Δ916-Npra in COS-7 cells resulted in a release of approximately 70% of¹²⁵I-ANP in culture media, whereas only 30% of¹²⁵I-ANP was released into culture media from COS-7 cells expressing the Δ635-Npra. Complete deletion of both KHD and guanylyl cyclase catalytic domain of Npra abolished the release of internalized ¹²⁵I-ANP into culture media. Interestingly, most of the internalization signals have been reported to reside in the cytoplasmic domains of endocytosed receptors (Parez et al., 1993; Sorokin et al., 1994; Haft et al., 1994; Huang et al., 1995). Previous studies have indicated that intracellular guanylyl cyclase catalytic domains of natriuretic peptide receptors (Npra and Nprb) are linked to a KHD-dependent mechanism that probably controls the guanylyl cyclase catalytic activity and the production of intracellular cGMP (Koller et al., 1992; Duda et al., 1993; Jewett et al., 1993). It has been suggested that KHD is critical for receptor function; however, the exact mechanism by which it controls the guanylyl cyclase catalytic activity or ligand-binding affinity of the receptor has not been clearly established. Our results demonstrate that sequential deletion of aa residues at the carboxyl-terminal end consisting of KHD and guanylyl cyclase catalytic domain of Npra determine the ligand-binding affinity, generation of second-messenger cGMP, and the metabolic turnover of ligand-receptor complexes in COS-7 cells.

Our deletion mutagenesis strategy has allowed us to alter selectively and sequentially the carboxyl-terminal end of the receptor to examine the structure-function relationship of Npra in terms of its binding affinity, catalytic activation, and trafficking of ligand-receptor complexes in COS-7 cells. These findings demonstrate that the specific sequence regions within the carboxyl-terminal domains of Npra determine the multiple functional properties of the expressed receptor protein, namely the extent of ligand-binding efficiency, generation of second-messenger cGMP, and the internalization and sequestration of ligand-receptor complexes in the intracellular compartments of intact COS-7 cells.