Identification and Characterization of the Prolactin-binding Protein in Human Serum and Milk*

J. Bradford Kline and Charles V. ClevengerDagger

From the Department of Pathology and Laboratory Medicine, University of Pennsylvania Medical Center, Philadelphia, Pennsylvania 19104

Received for publication, December 29, 2000, and in revised form, May 1, 2001


    ABSTRACT
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The actions of prolactin (PRL) are mediated by its receptor, a member of the superfamily of single transmembrane cytokine receptors. High affinity binding proteins for the closely related growth hormone have been found in the sera of several species including humans and are generated by alternative splicing or proteolysis of the growth hormone receptor extracellular domain (ECD). In contrast, no conclusive evidence has been presented that an analogous prolactin-binding protein (PRLBP) is expressed in human serum. Using both monoclonal and polyclonal antibodies generated against hPRL and the ECD of the human prolactin receptor, co-immunoprecipitation analyses of human serum identified a 32-kDa hPRLBP capable of binding both hPRL and human growth hormone. A measurable fraction of circulating PRL (36%) was associated with the hPRLBP. Despite well documented sex differences in serum hPRL levels, there were no significant differences in the levels of hPRLBP found in the sera of normal adult males and females (15.3 ± 1.3 ng/ml versus 13.4 ± 0.8 ng/ml, respectively (mean ± S.E.)). Immunoprecipitation studies also detected the PRLBP in human milk albeit at lower concentrations than found in sera. Deglycosylation did not alter its electrophoretic mobility, indicating an absence of carbohydrate moieties and suggesting that the hPRLBP spans most of the PRLR ECD, a result confirmed by limited proteolysis and mass spectrometry. The potential function of this serum chaperone was assessed in vitro by the addition of recombinant hPRLBP to the culture medium of the PRL-dependent Nb2 T-cell line. These studies revealed that the hPRLBP antagonizes PRL action, inhibiting PRL-driven growth in a dose-dependent manner.


    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Prolactin and growth hormone receptors are members of the cytokine receptor superfamily. Both the prolactin receptor (PRLR)1 and growth hormone receptor (GHR) are single-chain transmembrane proteins composed of an extracellular, transmembrane, and intracellular domain. The hormones prolactin (PRL) and growth hormone (GH) exert their effects at the molecular level by inducing the homodimerization of their respective receptors, initiating the activation of receptor-associated kinases and signaling cascades.

Until the last few decades, it was believed that peptide hormones circulated freely, but experimental evidence has proven otherwise. Although PRL was found to associate with serum IgG (1), a GH-binding factor was initially identified in the serum of pregnant mice (2) and subsequently discovered in rabbit (3) and human sera (4, 5). With the subsequent cloning of the GHR cDNA, a GH-binding protein (GHBP) was found to have amino acid sequence identity with the extracellular domain of the membrane-bound GHR (6). The GHBP is a 246-residue glycoprotein with a molecular mass of 50-60 kDa. The generation of GHRBP occurs via two separate mechanisms in mammals. In the mouse and rat, alternative splicing of a primary RNA transcript generates a truncated receptor in which the transmembrane domain is replaced by a short hydrophilic sequence (7-9). In other species, such as humans and rabbits, a full-length GHR is expressed, but GHBP is generated by proteolytic cleavage of the extracellular domain (6, 10, 11).

To date, although proteins in milk and serum have been found to interact with PRL, the existence of a free PRLR extracellular domain (ECD), i.e. a PRLBP, has not been established. Evidence for PRL-binding proteins in milk has been shown within humans (12, 13) as well as pigs, sheep, and rabbits (13, 14). Although the identity of two serum PRL-binding proteins has been recently established, namely IgG (1, 15) and cyclophilin B (16), no clear evidence exists for a PRLBP in mammalian serum (14, 17).

In this study, we characterize a PRLBP in human serum with identity to the ECD of the PRLR. The serum PRLBP was immunoreactive with both poly- and monoclonal antibodies generated against the extracellular domain of the PRLR and shows a proteolytic profile similar to a recombinant PRLR extracellular domain. Tryptic digest mass spectrometry (MS) further confirmed identity with the PRLR ECD. Coimmunoprecipitations revealed the association of the PRLBP with both serum PRL and GH. Furthermore, unlike the GHBP, the serum PRLBP is not glycosylated. Based on its PRL binding ability, it was also shown to inhibit the hormone-induced proliferation of Nb2 cells.

    EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Sera and Milk Samples-- Human sera were obtained from healthy male and female adult donors. Aliquots were stored at -80 °C and clarified by centrifugation at 12,000 × g for 30 min before use. Human milk was obtained from a lactating mother and defatted by centrifugation. Infranatant was collected by avoiding the upper lipid layer as well as any sediment and stored at -80 °C.

Expression of Recombinant Human Prolactin-binding Protein (rhPRLBP)-- A cDNA fragment of the human long PRLR was amplified by polymerase chain reaction with primers homologous to the mature form of the extracellular domain. The primers PRLR-1 (5'-CGAATTCCAGTTACCTCCTGGA-3') and PRLR-211' (5'-GCTCGAGTCATGTATCATTCATGGT-3') were used in the 50-µl amplification reaction with 50 ng of DNA template, 5 µl of 10 × polymerase chain reaction buffer, 3 µl of 25 mM MgCl2, 1 µl of 10 mM dNTP mix, and 5 units of Taq polymerase (Life Technologies, Inc.). After a 2-min incubation at 94 °C, the mixture was amplified for 30 cycles of 94 °C for 30 s, at 47 °C for 30 s, and at 72 °C for 30 s. It was then extended at 72 °C for 2 min. The amplified fragment was purified and concentrated by phenol/chloroform extraction followed by ethanol precipitation. The pellet was resuspended in 40 µl of dH2O, and 10 µl of the sample was digested with EcoRI and XhoI restriction enzymes and ligated into the corresponding restriction sites of pGEX4T-1 (Amersham Pharmacia Biotech). The clone was subsequently checked for amplification errors by dideoxynucleotide sequencing. The resulting glutathione S-transferase (GST)-ECD was expressed as per kit instructions. Briefly, a 1-liter culture of Escherichia coli transformant was grown to mid-log phase and induced with 0.1 mM isopropyl-1-thio-beta -D-galactopyranoside for 4 h. Pelleted cells were suspended in 20 ml of 10 mM EDTA and 10 mM Tris-HCl, pH 8.0, in the presence of 0.5 mg/ml lysozyme. Purification and solubilization of refolded GST-ECD was then carried out as described previously (18). For purification of bioreactive recombinant human PRLBP (rhPRLBP), 1 ml of refolded GST-ECD preparation was incubated with 300 µl of glutathione beads for 30 min at 4 °C. After washing the beads three times with PBS, protein was eluted in 300 µl of PBS containing 10 mM reduced glutathione. Thrombin protease (10 units) (Amersham Pharmacia Biotech) was added to the elution at room temperature for 18 h. The digested protein solution was dialyzed overnight in 4 liters of PBS and cleared of GST protein by three incubations with fresh glutathione beads. The purified rhPRLBP was electrophoresed on a 12% SDS-polyacrylamide gel and stained with Coomassie Blue to ensure the complete removal of GST protein as well as undigested fusion protein. The sample was incubated for 1 h with polymyxin beads to remove residual lipopolysaccharide and then filter-sterilized, aliquoted, and flash frozen.

Immunoprecipitation of PRLBP and PRL from Serum and Milk-- Sera and milk samples (1 ml) were thoroughly precleared of endogenous immunoglobulin by repeated overnight incubation with 300 µl of a protein A/G bead mixture. Precleared samples were then incubated overnight at 4 °C with 5 µl of rabbit anti-PRLR antiserum developed by our laboratory and characterized elsewhere (19). As a negative control, an equal aliquot of serum was incubated with 5 µl of normal rabbit serum. Immune complexes were then precipitated by the addition of 50 µl of protein A beads for 30 min at 4 °C. After three washes with lysis buffer (20 mM Tris-HCl, pH 7.5, 150 mM NaCl, 2 mM EDTA, 1% Triton X-100, 1 mM benzamidine, 1 mM phenylmethylsulfonyl fluoride, 1 mM Na3VO4, and 10 µg/ml aprotinin, pepstatin, and leupeptin), the beads were suspended in 30 µl of Laemmli buffer with mercaptoethanol and boiled. For the immunoprecipitation of serum PRL, samples were treated in a similar manner except that 5 µl of goat anti-PRL antiserum (Santa Cruz Biotechnology, Inc., Santa Cruz, CA) and 50 µl of protein G beads were used. For coimmunoprecipitation of GH with PRLBP, samples were immunoprecipitated with 5 µl of rabbit anti-PRLR antiserum plus 50 µl of protein A beads, washed three times, and suspended in Laemmli buffer as stated above.

Immunoblot Analysis-- Immune complexes were resolved by electrophoresis through a 12% SDS-polyacrylamide gel and transferred to polyvinylidene difluoride membrane (Bio-Rad). Nonspecific binding was blocked with 5% milk in PBS/Tween 20. Antigens were labeled with 1:1000 dilutions of primary antibodies and 1:2500 dilutions of horseradish peroxidase-coupled secondary antibodies. Antigen-antibody complexes were visualized by enhanced chemiluminescence (Amersham Pharmacia Biotech). Anti-PRLR antiserum used was described previously (19). Anti-PRLR monoclonal antibody directed against the human PRLR ECD was the gift of Genzyme, Inc. (Cambridge, MA). Rabbit anti-growth hormone antiserum was obtained from the National Institute of Diabetes and Digestive and Kidney Diseases.

Quantitation of Serum PRLBP, PRL, and GH-- To assess the quantities of PRLBP, PRL, and GH found in sera, immune complexes were electrophoresed in parallel with known quantities of recombinant human PRLBP, hPRL, or hGH. Visualized bands were then scanned, and signal intensities were obtained using ImageQuant densitometry software (Molecular Dynamics, Inc., Sunnyvale, CA). These data were used to generate a concentration/intensity curve to quantitate unknown amounts of PRLBP, PRL, or GH. Statistical analyses were performed using GraphPad Prism version 3.00 for Windows (GraphPad Software©, San Diego, California).

Deglycosylation of Serum PRLBP-- PRLBP was immunoprecipitated overnight with 5 µl of anti-PRLR antiserum and 50 µl of protein A beads as described above. Immune complexes were washed three times with lysis buffer, followed by three washes with 50 mM sodium phosphate, pH 7.5. Pellets were resuspended in 40 µl of 50 mM sodium phosphate with or without 10 units of glycopeptidase F (Sigma) and incubated for 8 h at 37 °C. Samples were washed once more with lysis buffer, resuspended in 40 µl of Laemmli buffer, and boiled. The treated and untreated samples were electrophoresed in parallel with 30 ng of recombinant PRLBP on a 12% SDS-polyacrylamide gel. This served as a control for the electrophoretic mobility of nonglycosylated PRLBP on a reducing gel. Samples were transferred to polyvinylidene difluoride and blotted with anti-PRLR mAb.

In-gel Protease Digestion of PRLBP-- Precleared serum (15 ml) was immunoprecipitated with 15 µl of anti-PRLR antiserum as described above, electrophoresed, and stained with Coomassie Brilliant Blue (Bio-Rad). After extensive destaining with 45% methanol, 10% acetic acid, the gel was washed with distilled water with several changes. The bands corresponding to the PRLBP were excised with a razor blade and suspended in 0.1 ml of 100 mM ammonium carbonate. Asp-N or Lys-C protease (Sigma) was added (1:25 w/w), and the mixture was thoroughly macerated with a microcentrifuge pestle (Kontes, Vineland, NJ). After overnight digestion at 37 °C, peptide fragments were separated from the gel pieces by centrifugation for 5 min at 2000 × g through a 1.5-ml low protein-binding microfilterfuge tube. Tricine sample buffer was added to the collected samples in the flow-through, boiled for 2 min, and separated on a 20% Tris-Tricine polyacrylamide gel. Bands were visualized using the Silver Stain Plus kit (Bio-Rad) per manufacturer's instructions and analyzed using the Scion Image for Windows densitometry software package (Scion, Inc., Frederick, MD).

Mass Spectrometry-- To isolate pure PRLBP from serum, covalently coupled anti-PRLR beads were generated for immunoprecipitation. Briefly, 200 µl of affinity-purified anti-PRLR antiserum was coupled to 100 µl of protein A beads for 1 h at room temperature. Beads were washed two times with 10 volumes of 0.2 M sodium borate (pH 9.0) and resuspended in 10 volumes of 0.2 M sodium borate, 20 mM dimethyl pimelimidate (pH 9.0) for 30 min at room temperature. Beads were washed in 0.2 M ethanolamine (pH 8.0) and then incubated for 2 h at room temperature in 0.2 M ethanolamine. The covalently coupled anti-PRLR beads were washed three times in PBS and mixed with 10 ml of precleared human serum overnight at 4 °C. The beads were then washed three times in 10 mM phosphate buffer (pH 6.8), and bound protein was eluted in 5 M LiCl, 10 mM phosphate buffer (pH 7.2). Sample was mixed with Laemmli buffer, boiled, and electrophoresed on a 10% SDS-polyacrylamide gel. The gel was stained with Silver Stain Plus (Bio-Rad), and the band corresponding to the PRLBP was excised for mass spectrometry. Samples corresponding to a plain gel slice and rhPRLBP were excised for use as negative and positive controls, respectively. The gel slices were subjected to in-gel tryptic digestion by rehydrating with 200 ng of sequencing grade trypsin (Promega, Madison, WI). Extractable tryptic peptides were subjected to MALDI-MS analysis using a paracrystalline film matrix method for desalting the extracts. Monoisotopic mass lists for the samples were generated and submitted for mass data base searching using the Profound algorithm (Rockefeller University, New York, NY).

Inhibition of Nb2 Lymphoma Cell Proliferation with Recombinant PRLBP-- Nb2-11C cells were maintained in Fisher's medium supplemented with 10% FCS, 10% horse serum, 1 mM L-glutamine, 100 units/ml penicillin, 100 µg/ml streptomycin, and 0.1 mM beta -mercaptoethanol. To assess the ability of recombinant hPRLBP to inhibit PRL-induced cellular proliferation, 1 × 104 Nb2 cells were aliquoted in triplicate wells in medium consisting of Dulbecco's modified Eagle's medium (Life Technologies, Inc.) supplemented with sodium selenide, linoleic acid, insulin, and transferrin (ITS+; Calbiochem) in the presence or absence of 50 pM hPRL, hPL, or hGH. Increasing concentrations (0-100 nM) of recombinant hPRLBP or 100 nM hPL, hGH, or BSA were simultaneously added to the wells. After overnight culture, cells were pulsed with 1 µCi of [3H]thymidine at 37 °C for 4 h. The incorporation of radiolabel was determined by scintillography of the harvested, washed cells.

    RESULTS
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Expression of a PRLBP in Human Serum-- To date, no protein with homology to the PRLR ECD has been found in sera, and the existence of such a protein in milk has been only indirectly implicated (12-14). This may in part be attributable to the absence of high avidity anti-PRLR antibody commercially available. Using a recently characterized anti-PRLR antiserum (19) in conjunction with a monoclonal antibody, we revisited the existence of a bona fide PRLBP (i.e. the free PRLR ECD) in human serum. To that end, human serum extensively precleared of immunoglobulin was immunoprecipitated with antiserum raised against the extracellular domain of the PRLR. Immunoblot analysis of this precipitate with a specific anti-PRLR mAb shows that the immunoprecipitate contained an immunoreactive protein corresponding to the approximate molecular weight of the extracellular domain of the human PRLR (Fig. 1A). This band was absent in the control lane using normal rabbit serum for the immunoprecipitation, illustrating the immunospecificity of the anti-PRLR antiserum. To quantitate the amount of PRLBP in the donor serum, the immunoprecipitation was repeated, and immunocomplexes were electrophoresed in conjunction with known quantities of recombinant PRLR (rPRLR) ECD (Fig. 1B). To ensure complete precipitation of PRLBP, the serum was used in a second round of immunoprecipitation (Fig. 1B, lane 3), revealing that the first immunoprecipitation had concentrated nearly all of the serum PRLBP. By comparison to the rPRLR ECD standards, it was determined that the donor had 13.8 ± 1.4 ng (mean ± S.E.) of PRLBP/ml of serum.


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Fig. 1.   PRLBP is expressed in human serum. A, immunoprecipitation of PRLBP from serum. Samples (1 ml) of precleared serum were immunoprecipitated in 5 µl of normal rabbit serum (NRS) or anti-PRLR antiserum overnight at 4 °C. After washing, precipitates were analyzed by immunoblot using anti-PRLR mAb (1:1000). An E. coli-expressed fusion of the hPRLR ECD to GST (GST-ECD) served as a positive control for antibody specificity. These results are representative of one of three experiments. B, quantitation of PRLBP in human serum. PRLBP was immunoprecipitated from serum as in panel A. To ensure the complete precipitation of PRLBP, serum was immunoprecipitated a second time (2°alpha -PRLR). Immunoprecipitates were electrophoresed in parallel with known quantities of recombinant PRLBP. Amounts of PRLBP in serum were calculated based on densitometry quantitation of standards. These results are representative of one of three experiments.

The Serum PRLBP Binds Serum PRL and GH-- Unlike any other species, hGH has the capacity to bind both the PRLR and GHR. Indeed, previous studies have shown that a milk PRL-interacting protein and GHBP are both capable of binding radiolabeled hGH (14). To determine whether there is an association between hPRL or hGH and PRLBP in human serum, coimmunoprecipitations were performed. As shown in the top panel of Fig. 2A, anti-PRLR immunoblot analysis of anti-PRL immunoprecipitates revealed the association of the PRLBP with serum PRL. Stripping and reprobing the blot with anti-PRL antibody shows that the immunoprecipitating antiserum was specific for PRL (Fig. 2A, bottom panel). As shown in Fig. 2B, anti-GH immunoblot analysis of anti-PRLR immunoprecipitates revealed that hGH was also bound to the PRLBP. To quantitate the amount of serum PRL complexed with PRLBP, immunoprecipitations were performed using anti-PRLR and anti-PRL antisera followed by immunoblotting with anti-PRL antiserum in conjunction with known concentrations of a PRL standard. As shown in Fig. 2C, 28 ng of PRL was found in 1 ml of a donor's serum, of which 10 ng or 36% coimmunoprecipitated with PRLBP as determined by known quantities of PRL electrophoresed in parallel. By similar methods, the amount of serum GH coimmunoprecipitating with PRLBP was analyzed. In this donor's serum, 2.6 ng of the 5 ng of GH present in 1 ml of serum associated with PRLBP (data not shown). To further investigate the PRL binding properties of the PRLBP, a recombinant form of the PRLBP was generated in E. coli for subsequent analysis by surface plasmon resonance. Using various concentrations of rPRLBP, the dissociation constant (Kd) of binding site I was measured at 13.4 nM, an observation similar to those reported in depth elsewhere2 and in good agreement with existing biosensor data (21).


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Fig. 2.   PRLBP associates with PRL and GH in human serum. A, association of serum PRL with PRLBP. Precleared serum was immunoprecipitated with normal rabbit serum (NRS) or goat anti-PRL antiserum (alpha -PRL). Immunoprecipitates were subjected to immunoblot analysis with alpha -PRLR mAb (top panel). The blot was stripped and reprobed with a 1:1000 dilution of alpha -PRL antiserum to ensure the immunoreactive specificity of the antiserum (bottom panel). These results are representative of one of three experiments. B, association of serum GH with PRLBP. Precleared serum was immunoprecipitated with normal rabbit serum or anti-PRLR antiserum (alpha -PRLR), and immunoprecipitates were subjected to immunoblot analysis with a 1:1000 dilution of alpha -GH antiserum (top panel). The blot was stripped and reprobed with a 1:1000 dilution of alpha -PRLR mAb (bottom panel). These results are representative of one of two experiments. C, quantitation of PRL bound to PRLBP in serum. Precleared serum samples (1 ml) were immunoprecipitated overnight with anti-PRLR, anti-PRL, or normal rabbit serum. Immunoprecipitates were electrophoresed in conjunction with known quantities of recombinant hPRL to determine the percentage of serum PRL complexed with PRLBP. These results are representative of one of two experiments.

Both Sexes Have Comparable Levels of Serum PRLBP-- Because the previous experiments utilized the serum of a single, nonlactating female donor, we wished to examine the variation in the levels of PRLBP observed between the sexes. This was accomplished by anti-PRLR immunoprecipitation analysis of donor serum and milk. As shown in Fig. 3, there was no significant difference in the amounts of PRLBP found in the sera of nonpregnant, nonlactating females (lanes 1-5) and males (lanes 6-9) with respective levels averaging 15.3 ± 1.3 ng/ml versus 13.4 ± 0.8 ng/ml PRLBP. We also observed no significant difference in the amounts of PRLBP found in the sera of these women as compared with sera from 24-h postpartum mothers (data not shown). Additionally, PRLBP was found in the breast milk of a lactating mother (Fig. 3A, lane 10) although at somewhat lower levels than in serum, as was similarly shown for other mammals (13, 14).


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Fig. 3.   PRLBP is expressed in the sera of both males and females. A, immunoblot of serum samples. Precleared sera samples and breast milk were immunoprecipitated with alpha -PRLR antiserum and subjected to immunoblot analysis with a 1:1000 dilution of anti-PRLR. B, quantitation of PRLBP in the sera of both sexes. Bands from panel A were analyzed by densitometry against known quantities of recombinant PRLBP to quantitate the amounts of PRLBP found in serum. Males, 15.3 ± 1.3 ng/ml; females, 13.4 ± 0.8 ng/ml (mean ± S.E.). NRS, normal rabbit serum.

Biochemical Identification of the PRLBP-- The PRLR is known to be highly glycosylated on the asparagine residues of its extracellular domain (22). To determine whether the PRLBP was glycosylated to a similar degree, immunoprecipitated PRLBP was treated with the general deglycosidase glycopeptidase F and then electrophoresed along with recombinant PRLBP expressed in E. coli (Fig. 4A). No shift in electrophoretic mobility was observed upon glycopeptidase F treatment, suggesting that serum PRLBP was not glycosylated and had the same apparent molecular mass as the recombinant form of the PRL ECD (32 kDa). Although two antibodies generated against the extracellular domain of the PRLR were immunoreactive against serum and milk PRLBP (Figs. 1 and 2), we could not entirely rule out that this was attributable to cross-reactivity to a highly homologous protein. Attempts at N-terminal amino acid sequencing, however, were noninformative, possibly because of a blocked N terminus. Therefore, serum PRLBP was excised from an SDS-polyacrylamide gel and subjected to protease digestion with Asp-N or Lys-C (Fig. 4B). As a positive control, recombinant PRLR ECD was digested in parallel. GST digestion served as a negative control. The peptide fragments resulting from the digestion of serum PRLBP showed an electrophoretic profile highly similar to the PRLR ECD (Fig. 4B, row 1 versus row 2). In contrast, the pattern differed from that of GST (Fig. 4B, row 2 versus row 3), suggesting that the PRLBP was indeed homologous to the extracellular domain of the PRLR. To confirm this observation, MALDI-MS was performed on PRLBP immunoprecipitated from serum as compared with recombinant human PRLBP. Four tryptic peptides with molecular masses of 971, 1399, 1772, and 1893 correlated between the serum PRLBP and the positive control of rPRLR ECD (Fig. 4C, middle versus bottom panel). Mass data base searching revealed homology to the PRLR ECD, and two peaks corresponded to tryptic fragments of this region (Fig. 4C, arrows in the bottom panel).


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Fig. 4.   Biochemical characterization of the PRLBP. A, PRLBP is not glycosylated. Precleared serum was immunoprecipitated with anti-PRLR antiserum, and the immunoprecipitate was washed and incubated with or without 10 units of glycopeptidase F (PNGase F) in buffer for 8 h at 37 °C. Samples were immunoblotted in parallel with recombinant PRLBP and probed with a 1:1000 dilution of anti-PRLR mAb. B, proteolytic analysis of serum PRLBP versus PRLR ECD. Serum was immunoprecipitated with anti-PRLR antiserum as described above, electrophoresed, and stained with Coomassie Brilliant Blue. Excised bands were digested with Asp-N and Lys-C, and peptide fragments were separated on a 20% Tris-Tricine polyacrylamide gel. Bands were visualized using the Silver Stain Plus kit (Bio-Rad) and scanned for densitometric analysis. Recombinant PRLR ECD served as a positive control, and GST served as a negative control. These results are representative of one of two experiments. C, MALDI-MS identification of the hPRLBP. Serum was immunoprecipitated with protein A beads covalently linked to anti-PRLR antibodies. Eluted hPRLBP was electrophoresed and stained with Silver Stain Plus (Bio-Rad). Excised bands were digested with trypsin and subjected to MALDI-MS. Two peptides corresponding to the ECD of the human PRLR are indicated. rECD, recombinant ECD; pT, trypsin autolysis product; TOF, time of flight; LD, limit of detection.

Recombinant Human PRLBP Inhibits the Proliferation of Nb2 cells Stimulated with Human PRL-- As the GHBP can modulate the activity of GH, we wished to determine the effect of purified recombinant PRLBP on the biological activity of hPRL using the rat Nb2-11C lymphoma cell proliferation assay (Fig. 5). As increasing concentrations of PRLBP were added, a 3-fold reduction in cell proliferation was noted (Fig. 5A). Importantly, the PRLBP by itself was not toxic to cells. Therefore, the overall decrease in proliferation could be attributed to the PRLBP competing with cell surface receptors for ligand. This competition also extended to other members of the somatolactogenic family of ligands. As the control protein BSA was observed to have no positive or negative effect on PRL-induced proliferation (data not shown), we compared the effects of coincubation of BSA or PRLBP with other somatolactogenic hormones on Nb2 cell proliferation. The inclusion of PRLBP into the medium of either PL- or GH-stimulated Nb2 cells was found to decrease ligand-induced cell proliferation, an effect not observed for BSA (Fig. 5B).


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Fig. 5.   Effect of rhPRLBP on the proliferation of Nb2 lymphoma cells. A, rhPRLBP blocks hPRL-induced Nb2 cell proliferation in a dose-dependent manner. 1 × 104 cells were plated overnight in Dulbecco's modified Eagle's medium/ITS+ supplemented with 50 pM hPRL and increasing concentrations of hPRLBP. Proliferation was assessed by tritiated thymidine uptake. Results are mean disintegrations/min (DPM) of triplicate wells ± S.E. B, rhPRLBP blocks Nb2 cell proliferation induced by hPL and hGH. 1 × 104 cells were plated overnight in Dulbecco's modified Eagle's medium/ITS+ supplemented with 50 pM hPRL, hPL, or hGH in conjunction with 100 nM rhPRLBP or 100 nM BSA. Proliferation was assessed by tritiated thymidine uptake. Results are mean disintegrations/min of triplicate wells ± S.E.


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Previous searches for the presence of a soluble form of the PRLR in mammalian biological fluids only resulted in the discovery of a putative PRLBP in milk samples (12-14). However, attempts to find a PRLBP in sera were unsuccessful, resulting from the general lack of robust anti-PRLR antibodies. In this study, we show evidence for a soluble PRLBP in human plasma. Using a high avidity anti-PRLR antiserum (19) generated by our laboratory, it was possible to immunoprecipitate a protein from human plasma that was subsequently recognized by an anti-PRLR monoclonal antibody during immunoblot analysis (Fig. 1A). This serum PRLBP was observed to have the same molecular mass (32 kDa) as the extracellular domain of the human PRLR expressed in E. coli and was not glycosylated based on the inability of a glycosidase to affect its electrophoretic mobility (Fig. 4A). Our findings extend an observation by Mercado and Baumann (12) in which a PRL-binding protein in milk bound to hGH affinity columns, but unlike the GHBP in human plasma, did not bind to wheat germ lectin columns, suggesting an absence of glycosylation. However, this study was unable to confirm the immunological identity of this species as that of the PRLR ECD. Interestingly, the predicted molecular mass of rhPRLBP expressed in E. coli is 24.5 kDa, yet both native and recombinant forms migrate as 32-kDa proteins. This difference in the predicted and observed masses may be attributable to the high content of acidic and proline residues comprising the PRLBP (21%). Previous studies have reported this same discrepancy because of the retarded mobility of a variety of proteins based on proline and acidic residue content (23-25). To confirm the identity of the PRLBP with the PRLR ECD, the immunoprecipitated PRLBP was subjected to limited proteolysis and SDS-polyacrylamide gel electrophoresis analysis alongside similarly digested rhPRLR ECD (Fig. 4B). Both proteins exhibited similar peptide fingerprints from both digestions, further supporting the correlation between the PRLBP and the extracellular domain of the PRLR. Finally, MALDI-MS analysis and monoisotopic mass lists for the sample revealed homology with the PRLR by data base searching using the Profound algorithm. Although there were four identical peptides between rhPRLR ECD and serum PRLBP, two were found in the data base search to correspond to fragments of the PRLR ECD. It is probable that incomplete tryptic digestion of the samples would explain why the other two fragments were not identified in the data base search. Thus, given the existing precedent with the naming of the GHBP, we therefore have termed the serum protein identified in these studies as the PRLBP.

The mechanism for PRLBP generation as well as its tissue source is unknown. The generation of GHBP varies by species because rodents produce GHBP by alternative splicing mechanisms (7, 8, 26), whereas humans (6, 10) and rabbits (11) produce GHBP by the specific proteolysis of the membrane receptor. Indeed, Saito et al. (27) observed the constitutive release of GHBP from IM-9 cells. This was believed to be the result of surface GHR being cleaved by a metalloprotease because EDTA inhibited the production of GHBP. Membrane-bound PRLR is known to be N-link glycosylated (28), an event crucial for its cell surface targeting (22). The fact that a soluble, nonglycosylated PRLBP is present in milk and serum in humans therefore suggests that the binding protein may be produced by a combination of deglycosylation and proteolysis of the full-length PRLR. Indeed, although we observed the association of glycosylated full-length PRLR from T47D cell lysates with concanavalin A beads, neither rhPRLBP nor serum PRLBP was observed to bind to the beads (data not shown). This suggests that only the deglycosylated form of the PRLBP is found in serum. Interestingly, it has been shown that certain plasma membrane glycoproteins of hepatocytes undergo rapid deglycosylation (29, 30). As the liver abundantly expresses the PRLR (31), proteolytic cleavage of deglycosylated hepatic receptors could be one possible source of PRLBP in human serum. Current studies are underway to address this hypothesis.

The PRLBP was present in the sera of both males and females at comparable levels. This absence of sexual dimorphism is reminiscent of the PRLR itself (32). Like previous reports, which indicated that a protein capable of binding PRL was present in human milk (12, 14), our data would now indicate that this species represents the PRLBP. Additionally, the milk PRLBP was observed to be at a lower concentration than serum PRLBP, which is consistent with the observed levels of GHBP in human milk versus serum (12). Preliminary data from our laboratory suggest that there is no significant increase in serum PRLBP levels from mothers 24 h postpartum (data not shown). Interestingly, this is in direct contrast with the levels of GHBP observed during rodent gestation. In the mouse, increases in the levels of serum GHBP are observable on Day 9 of gestation, and by late gestation serum GHBP levels increase 30-fold (33). This may also be regulated by GH itself because continuous exposure to elevated GH in nonpregnant rats results in the up-regulation of GHBP (9, 34). In contrast, however, it is interesting to note that a pregnancy-associated rise in GHBP is not driven by GH (35).

Because the membrane-bound PRLR is capable of binding both PRL and GH, we wished to determine the ligand binding characteristics of the PRLBP. Surface plasmon resonance experiments for the hPRLBP were consistent with previously reported hormone-receptor interactions such as those observed by Gertler et al. (21). The PRLBP was found associated with both PRL and GH in human serum, and ~36% of plasma PRL was found associated with PRLBP in a single donor (Fig. 2). In a separate single donor, ~53% of plasma GH was found to be associated with the PRLBP. This result is similar to that observed with GHBPs because GHBPs complex 45-55% of circulating GH under basal conditions (36-38). This has been shown to slow the renal clearance of GH, thereby providing a longer lasting reservoir of hormone (39, 40). Quantitative analysis of the molar concentration of the PRLBP, GH, and PRL indicated that the PRLBP is nearly saturated with somatolactogenic hormone, suggesting that the ligand-bound PRLBP may serve as a significant buffer to hormone levels.

Although a decrease in the clearance of PRL by the PRLBP could enhance the activity of PRL in vivo, in vitro studies using recombinant hGHBP have shown that GHBP inhibits GH activity (41). Similarly, the bovine PRLR extracellular domain has been shown to inhibit the bioactivity of ovine PRL on Nb2 cells (42). Because the hPRLBP was capable of binding PRL, we wished to determine whether a recombinant form of the human PRLBP could inhibit the hPRL-induced proliferation of Nb2 cells (Fig. 5A). A dose-dependent decrease in Nb2 cell proliferation was observed when recombinant hPRLBP was added to cells. This was also observed in the presence of hPL and hGH (Fig. 5B), suggesting that the PRLBP is capable of binding these hormones as well. Although PRLBP was capable of inhibiting PRL-mediated cell proliferation in vitro, the effects of PRLBP in vivo may differ greatly. In a rat model, human GHBP complexed with hGH was cleared at a significantly slower rate, exhibited limited extravascular availability, and degraded at a slower rate than free hGH (39). Similarly, hypophysectomized rats given GH in conjunction with GHBP showed significantly greater growth and weight gain compared with animals given GH alone (20). Based on these findings, the in vivo presence of PRLBP may serve to maintain a reservoir of PRL in the circulation, providing a releasable pool of free hormone in times of diminishing supply.

    ACKNOWLEDGEMENTS

We thank David Goodman and Anne Crivaro for providing us with human sera samples. We thank William Moore for contributing to the MALDI-MS analysis.

    FOOTNOTES

* This study was supported in part by Grants 2R01CA69294 (to C. V. C.) and 1F32DK09727 (to J. B. K.) from the National Institutes of Health.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.

Dagger To whom correspondence should be addressed: Dept. of Pathology and Laboratory Medicine, University of Pennsylvania Medical Center, 513 Stellar-Chance Laboratories, 422 Curie Blvd., Philadelphia, PA 19104. E-mail: clevengc@mail.med.upenn.edu.

Published, JBC Papers in Press, May 3, 2001, DOI 10.1074/jbc.M011786200

2 J. B. Kline and C. V. Clevenger, submitted for publication.

    ABBREVIATIONS

The abbreviations used are: PRLR, prolactin receptor; PRL, prolactin; GH, growth hormone; GHR, growth hormone receptor; PRLBP, prolactin-binding protein; GHBP, growth hormone-binding protein; h, human; rh, recombinant human; r, recombinant; PL, placental lactogen; GST, glutathione S-transferase; ECD, extracellular domain; Tricine, N-[2-hydroxy-1,1-bis(hydroxymethyl)ethyl]glycine; MALDI-MS, matrix-assisted laser desorption/ionization-mass spectrometry; PBS, phosphate-buffered saline; BSA, bovine serum albumin; mAb, monoclonal antibody.

    REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

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