From the I. Medizinische Klinik, Abteilung Pathophysiologie,
Johannes Gutenberg-Universität Mainz, Obere Zahlbacher Strasse
63, D-55101 Mainz, Germany and the Institut für
Biochemie, Klinikum der RWTH Aachen, Pauwelsstrasse 30, D-52057
Aachen, Germany
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ABSTRACT |
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Interleukin-6 (IL-6) belongs to the family of the "four-helix bundle" cytokines. The extracellular parts of their receptors consist of several Ig- and fibronectin type III-like domains. Characteristic of these receptors is a cytokine-binding module consisting of two such fibronectin domains defined by a set of four conserved cysteines and a tryptophan-serine-X-tryptophan-serine (WSXWS) sequence motif. On target cells, IL-6 binds to a specific IL-6 receptor (IL-6R), and the complex of IL-6·IL-6R associates with the signal transducing protein gp130. The IL-6R consists of three extracellular domains. The NH2-terminal Ig-like domain is not needed for ligand binding and signal initiation. Here we have investigated the properties and functional role of the third membrane proximal domain. The protein can be efficiently expressed in bacteria, and the refolded domain is shown to be sufficient for IL-6 binding. When complexed with IL-6, however, it fails to associate with the gp130 protein. Since the second and the third domain together with IL-6 can bind to gp130 and induce signaling, our data demonstrate the ligand binding function of the third domain and point to an important role of the second domain in complex formation with gp130 and signaling.
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INTRODUCTION |
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Interleukin-6-type cytokines (IL1-6, IL-11, CT-1, CNTF, LIF, OSM) are cytokines with a characteristic helical fold (1, 2). All these cytokines act via receptor complexes, which contain at least one molecule of gp130, the common signal transducing protein of the IL-6 family of cytokines (2). IL-6 and IL-11 act via a homodimer of gp130, whereas CT-1, CNTF, LIF, and OSM require a heterodimer of gp130 and the related protein LIF-receptor (LIF-R) (2). Recently it has been shown that in the human system OSM additionally binds and acts via a receptor complex consisting of gp130 and the OSM receptor, a protein related to gp130 and LIF-R (3). In the murine system, the gp130 and OSM receptor complex seems to be the only complex that is bound and activated by OSM (4).
Interestingly, the cytokines IL-6, IL-11, CT-1, and CNTF first bind to their specific receptor proteins and induce intracellular signaling by subsequent association of this complex with a gp130/gp130 homodimer or a gp130/LIF-R heterodimer. In contrast, LIF and OSM bind directly to LIF-R and gp130, respectively, leading to the formation of heterodimeric gp130-LIF-R or gp130/OSM-R complexes (2). Thus, LIF and OSM do not require specific cytokine receptor subunits as do IL-6, IL-11, CT-1, and CNTF.
The three-dimensional structures of IL-6 (5), CNTF (6), and LIF (7) have been solved and have been shown to share a common "four-helix bundle" fold. The specific ligand binding receptors for IL-6, IL-11, and CNTF are membrane proteins, the extracellular parts of which consist of three domains. Cytokine binding occurs via the cytokine-binding module (CBM), which consists of the second (D2) and the third (D3) domains. The three-dimensional structure of the CBM domain of gp130 has recently been solved (8). It is structurally highly related to the extracellular parts of the growth hormone receptor (9), the prolactin receptor, and the erythropoietin receptor.
The specific receptors for IL-6, IL-11, CT-1, and CNTF cytokines exist in a membrane bound and a soluble form (10-13). In contrast to most soluble receptors for cytokines and growth factors, the soluble receptors of the IL-6 family complexed with their ligands can elicit a biological signal on cells that only express the signaling subunits gp130 and LIF-R. This process has recently been called transsignaling (14). Whereas virtually all cells of the body express gp130, the proteins LIF-R, IL-6R, CNTF-R, and IL-11R are only expressed on some cell types (2). Recently, it has been shown that cell types that respond exclusively to IL-6/sIL-6R, but not to IL-6 alone, include hematopoietic progenitor cells (15), endothelial cells (16), osteoclasts (17), and neuronal cells (18).
Structure-function analyses of the human IL-6R (19, 20) have shown that the NH2-terminal Ig-like domain of the receptor protein is not needed for ligand binding and biological activity. So far, the contribution of the single D2 and D3 domains to ligand binding and gp130 activation has not been analyzed. Here we show that the D3 domain alone is sufficient for IL-6 binding but cannot associate with gp130.
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MATERIALS AND METHODS |
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Chemicals--
Restriction enzymes were obtained from AGS
(Heidelberg, Germany). Vent polymerase was from New England Biolabs
(Beverly, MA). Isopropyl--D-thiogalactopyranoside was
purchased from GERBU (Gaisheim, Germany). Guanidine hydrochloride was
from Fluka (Buchs, Switzerland). The preparation of the polyclonal
monospecific antisera against IL-6R (6.2) was described previously
(21). Anti-rabbit IgG POD conjugate was purchased from Sigma
(Deisenhofen, Germany). Precipitating and soluble BM blue substrates
for detection of peroxidase activity were obtained from Boehringer
Mannheim (Mannheim, Germany). Skimmed milk powder was from ICN
(Meckenheim, Germany).
Construction of a D3 Expression Vector-- The D3-encoding region of the IL-6R-cDNA was amplified by PCR using an IL-6R-cDNA (22) as a template. NdeI and HindIII sites were introduced in the 5'- and 3'-primers, respectively, to enable cloning of the amplified DNA in the NdeI and HindIII sites of the procaryotic expression vector pRSET 5b (23, 24) (sense-primer, 5' CCG GCG CAT ATG GGA ATC TTG CAG CCT G 3'; antisense-primer, 5' GGC CCA AGC TTA AGT AGT AAG TGC CTG C 3'). PCR was performed in a total volume of 50 µl of PCR buffer (10 mM KCl, 20 mM Tris-HCl, pH 8.8, 10 mM (NH4)2SO4, 2 mM MgSO4, 0.1% Triton X-100, 0.2 mM of each dNTP) containing 0.25 ng of template DNA, 0.5 unit of Vent DNA-polymerase, and 1 µM D3 sense and antisense primer pairs, respectively. Amplification of D3 DNA by PCR was performed with 35 cycles of denaturation (45 s, 94 °C), primer annealing (45 s, 60 °C), and elongation (45 s, 72 °C). PCR products were purified, subsequently digested with NdeI and HindIII, and ligated into the pRSET 5b vector opened with NdeI and HindIII. The D3 cDNA construct was verified by restriction analysis and automated DNA sequencing.
Expression of D3 in Escherichia coli--
E. coli
BL21 (DE3) cells (23, 24) were transformed with the D3 expression
vector. 200 ml of minimal medium as has been described (25) were
supplemented with ampicillin (50 µg/ml), glucose (5 g/liter), and
trace elements (25), inoculated with a 2-ml culture of a single clone,
and cultured overnight at 37 °C. A biofermentor (BIOFLO 3000, New
Brunswick Scientific, Edison, NJ) was charged with 3 liters of minimal
medium, inoculated with the total overnight culture, and incubated at
37 °C and a minimum oxygen saturation of 30%. Expression of the
recombinant protein was induced by adding
isopropyl--D-thiogalactopyranoside (final concentration:
0.4 mM) at an A600 of about 3 when a
specific growth rate of µ = 0.7 was reached, and the fermentation
process was maintained for a further 2 h. Cells were harvested by
centrifugation and resuspended in lysis buffer (50 mM
Tris-HCl, pH 7.5, 1 mM EDTA, 1% Tween 20, 1 mM
dithiothreitol, 1 mM phenylmethylsulfonyl fluoride).
Complete lysis of bacteria was achieved by three freeze/thaw steps
followed by two cycles of sonification (3 min) and several cycles of
washing and centrifugation resulting in a preparation of purified
inclusion bodies. Supernatants and pellets were analyzed by SDS-PAGE
and Western blotting. Inclusion bodies were solubilized in 6 M guanidine HCl, 50 mM Tris-HCl, pH 8.0, 10 mM dithiothreitol.
Protein Purification and Refolding-- A Superdex200 (16/60) column (Amersham Pharmacia Biotech) was equilibrated with refolding buffer (50 mM sodium phosphate, pH 5, 250 mM NaCl, 1 mM dithiothreitol, 0.5 mM EDTA), loaded with 1.5 ml of solubilized inclusion bodies (200 µg of protein), and run with a constant flow rate of 1.5 ml/min. Fractions of 2 ml were collected, analyzed by SDS-PAGE, and significant fractions were pooled and concentrated. By this method 30 mg of purified protein were obtained from a single fermentation process (3 liters of bacterial culture).
CD Spectroscopy-- CD measurements were carried out on an Aviv (Aviv Associates, Lakewood, NJ) 62DS CD spectrometer equipped with a temperature control unit and a Jasco J-600 spectropolarimeter, both calibrated according to Chen and Yang (26). The spectral bandwidth was 1.5 nm. The time constant ranged between 1 and 4 s and the cell path length between 0.1 and 10 mm.
Western Blotting-- For detection of D3, purified protein or inclusion bodies from different purification steps were separated on 12.5% SDS-polyacrylamide gels and electroblotted onto nylon filters (GeneScreen Plus, NEN Life Science Products). Filters were blocked and incubated with polyclonal rabbit antibody to IL-6R 1:2000 followed by anti-rabbit IgG POD conjugate 1:2000. Peroxidase activity was detected using precipitating BM blue POD substrate.
D3 ELISA-- Binding of D3 to IL-6 was analyzed by sandwich ELISA at 22 °C. Purified recombinant IL-6 was coated on ELISA plate wells (Microtest III, Falcon, Oxnard, CA) at 10 µg/ml. After blocking of unspecific binding with PBS containing 5% skimmed milk powder, D3 was applied at 10 µg/ml. After washing, bound protein was detected with polyclonal rabbit antibody to IL-6R 1:2000 followed by anti-rabbit IgG POD conjugate 1:2000. Peroxidase activity was detected with soluble BM blue POD. In every ELISA, recombinant soluble IL-6R (consisting of D2 and D3), expressed in Pichia pastoris and purified as described previously (20), was applied in paralell at 10 µg/ml. For negative control the equivalent experiment was performed with the ELISA plate wells coated with PBS containing 5% skimmed milk.
Immunoprecipitation-- 100 ng of purified D3 protein or sIL-6R were incubated for 4 h at 4 °C with a 20-fold excess of human IL-6-Fc or a 10-fold excess of human gp130-Fc (alone or in combination with 300 ng of recombinant human IL-6) or a human IL6-sIL-6R fusion construct called H-IL-6-Fc (27).2 All Fc proteins were obtained from supernatants of transiently transfected COS-7 cells and purified via protein A affinity chromatography. Concentrations were checked using standard protein assays. Immune complexes were precipitated with protein A-Sepharose, separated on 12.5% SDS-polyacrylamide gels, and blotted as described above. Both precipitated D3 protein and sIL-6R again were detected using polyclonal rabbit antibody to IL-6R.
Kinetic Assay-- IL-6 was covalently immobilized to a carboxymethyl dextran matrix (Fisons, Loughborough, UK) at 2.25 µg/ml for 2 min in 10 mM sodium acetate buffer, pH 5.0, as recommended by the manufacturer (28). Binding experiments were performed at controlled temperature (25 °C) with 10 different concentrations of purified D3 protein using the IASYSTM (Fisons) optical biosensor. Association was monitored for at least 2 min, the sample was replaced by PBS/0.05% Tween 20 (PBST), and dissociation was monitored accordingly before the cuvette was regenerated with 5 mM HCl and equilibrated again in PBST. Association and dissociation affinograms were analyzed by nonlinear regression with the FASTfit (Fisons) software, which uses the Marquardt-Levenburg algorithm for iterative data fitting.
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RESULTS |
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Expression, Purification, and Refolding of D3-- For expression of D3 of IL-6R in E. coli, the respective cDNA fragment was amplified by PCR and cloned into the expression vector pRSET 5b (23, 24). The expressed protein consisted of D3 together with the epitope recognized by the antibody 6.2 (Fig. 1A) (21). After expression in a biofermenter and lysis of cells, the protein was exclusively found in inclusion bodies (IB). No recombinant protein was found in the supernatant of the inclusion bodies (SN IB). The expressed protein was visualized as a 17-kDa band by SDS-PAGE (Fig. 1B) and Western blotting (Fig. 1C). Refolding and purification of the highly enriched protein was achieved by solubilization of the inclusion bodies in guanidine hydrochloride and subsequent gel filtration on a Superdex200 column equilibrated with sodium phosphate buffer (29). Upon rechromatography of the refolded protein, a single peak was observed indicating that no dimers or higher aggregates were formed during the recovery process of D3 (data not shown).
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Structural Characterization of D3--
The folding state of the
protein was characterized by CD spectroscopy. Fig.
2A shows the far-UV CD
spectrum of D3. The spectrum was indicative of a protein in a folded
state. The prominent band at 232 nm is the positive lobe of a couplet,
which can be attributed to interacting tryptophan side chains (30). It
had also been observed in the far-UV CD spectrum of the corresponding
domain of the granulocyte-colony-stimulating factor receptor (31) and the third extracellular domain of gp130 (29). This band seems to be
characteristic of the WSXWS motif present in the
COOH-terminal domain of the CBM in all class I cytokine receptors.
Secondary structure analysis of the CD spectrum showed that the protein mainly consisted of -sheet (D3:
-sheet = 56%;
-helix = 0%), confirming the secondary structure prediction
(32). The folded state of the protein was also evident from the near-UV
CD spectrum (Fig. 3B), which
showed several distinct bands attributable to tyrosine and tryptophan
side chains (30). These data demonstrated that purification and
refolding of D3 from solubilized inclusion bodies could be achieved in
a one-step procedure using size-exclusion chromatography.
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Thermal Unfolding of D3-- The thermal stability of the molecule at pH 6.8 was also studied by CD spectroscopy. Fig. 3A shows a series of far-UV CD spectra recorded at different temperatures. With increasing temperature the prominent positive band at 232 nm decreases. The ellipticity at 232 nm was plotted as a function of temperature in Fig. 3B. The transition midpoint for D3 at pH 6.8 is 35 °C, indicating a remarkable thermal instability of this domain.
Binding of D3 to IL-6 as Detected by Sandwich ELISA-- We next asked whether D3 was able to bind human IL-6. IL-6 was immobilized to a 96-well ELISA dish, and binding was assayed by indirect ELISA as described under "Materials and Methods." D3 was recognized by the antibody 6.2 as efficiently as sIL-6R, as shown by Western blotting (Fig. 1C). In Fig. 4, measurements of D3 and of sIL-6R binding to IL-6 are shown. Binding of IL-6 by D3 and by sIL-6R (consisting of domains D2 + D3) (20) were comparable.
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Kinetics of Binding of D3 to IL-6--
When human IL-6 was
immobilized to an IAsysTM cuvette (see "Materials and
Methods") real-time interaction between IL-6 and D3 could be
analyzed. In Fig. 5A
association curves recorded for 10 concentrations of D3 are shown. For
clarity, dissociation, although measured for all concentrations, is
shown only for the highest concentration. The obtained data were used
to calculate an association rate, ka = 2.72 × 104 ± 1467.61 M1
s
1, and a dissociation rate, kd = 1.04 × 10
2 ± 0.0009 s
1, between IL-6
and D3. From these values an affinity of KD = 385 nM can be derived (Fig. 5B). For comparison,
reported affinities for the interaction of immobilized IL-6 and entire
soluble IL-6R (33) or the immobilized entire sIL-6R and IL-6 (34),
which also were mesured at controlled temperature (25 °C) (33, 34), were about 10-fold higher.
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Immunoprecipitation of D3 with IL-6-Fc-- We next asked whether binding of D3 to IL-6 could be detected in solution and whether a D3/IL-6-complex was able to associate with the signal transducing protein gp130. To answer these questions we incubated purified D3 protein with Fc fusion proteins of IL-6 and gp130 in the presence or absence of IL-6. We have recently constructed a fusion protein consisting of human IL-6 and human soluble IL-6R in which both proteins were covalently linked by a flexible polypeptide linker (27). This fusion protein was called Hyper-IL-6 (H-IL-6). This IL-6/sIL-6R fusion protein was expressed as an Fc fusion protein (H-IL-6-Fc). Since we have shown that in the H-IL-6 fusion protein, the IL-6R binding site of IL-6 is not accessible for free IL-6R (27), this H-IL-6-Fc protein was used as a negative control. Bound protein was immunoprecipitated and detected by Western blotting. As shown in Fig. 6A, D3 could be precipitated with IL-6-Fc (left lane), but not with the combination of IL-6 and gp130-Fc. There was no binding of D3 to gp130-Fc alone or to H-IL-6-Fc. In Fig. 6B the identical experiment is shown using the sIL-6R consisting of D2 and D3, which could be precipitated with both, IL-6-Fc, and the combination of IL-6 and gp130-Fc. Interestingly, the sIL-6R was almost quantitatively precipitated by IL-6-Fc, whereas only 5-10% of the D3 protein was captured by IL-6-Fc, possibly reflecting the lower affinity of D3 for IL-6 (see above). These results clearly show that D3 of sIL-6R, although being able to bind IL-6, could not mediate an association of the complex with gp130.
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DISCUSSION |
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Four conclusions can be drawn from our study: (i) the third domain of the human IL-6R can be expressed on its own and correctly refolds in vitro. (ii) The protein is remarkably unstable to thermal perturbation. (iii) D3 on its own binds the ligand IL-6, albeit with a lower affinity than the complete human IL-6R. (iv) Although D3 is sufficient for IL-6 binding, the complex of D3 and IL-6 fails to associate with gp130.
Receptors for the four-helix cytokines have been shown to be composed of Ig and fibronectin type III-like domains (35). Specific ligand recognition has been ascribed to the CBM, which consists of two of such fibronectin type III-like domains defined by a set of four conserved cysteines and a tryptophan-serine-X-tryptophan-serine (WSXWS) sequence motif (32). In the case of the growth hormone-growth hormone receptor complex, it has been demonstrated that both domains of the CBM are involved in ligand binding (9).
The extracellular portion of human IL-6R consists altogether of three
domains (22). The NH2-terminal domain has been shown to be
dispensable for ligand recognition and signal initiation (19, 20).
Recent experiments might point to a role of the NH2-terminal domain of the IL-6R for intracellular
processing and protein
stability.3 Ligand
recognition by the CBM of human IL-6R is believed to occur via the
loops which connect the -strands within the two fibronectin type
III-like domains (36). In analogy to the growth hormone-growth hormone
receptor complex, the third domain of IL-6R is predicted to establish a
contact with the respective domain of the CBM of gp130 (36). In fact,
mutations in a membrane proximal loop region of the IL-6R, which was
predicted to be involved in such a contact, turned out to prevent
association of the IL-6·IL-6R complex with gp130 (37). Such IL-6R
muteins turned out to be weak antagonists of IL-6 (37).
Our results demonstrate that D3 of human IL-6R on its own is sufficient for ligand binding. The affinity we measured is about 1 order of magnitude lower than the one determined for the entire sIL-6R (33, 34). As suggested by our model of the IL-6·IL-6R complex (36), there are two contact regions between IL-6 and IL-6R. The D2 portion of IL-6R is in contact with the 2c region (loop between the helix A and the helix B) (38). The D3 portion of the IL-6R touches the COOH-terminal part of helix D, which also has been implicated in receptor binding (39, 40). A possible explanation for the low affinity between D3 and IL-6, which we observed in this study, is that loop residues of D2 contribute to ligand binding and thereby to the affinity of the IL-6R (36). As discussed above, D3 was shown to be essential for the contact between IL-6R and gp130. Our data demonstrate that this contact is not sufficient for association of the D3·IL-6 complex with gp130. This implies that D2 is needed for the formation of the complex between IL-6, IL-6R, and gp130.
We have shown that D3 of the human IL-6R has a remarkably low thermal stability. Unfolding starts already at 28 °C. For comparison, the analogous domain of gp130 is stable up to 34 °C. One consequence of this instability of D3 is that this protein does not exhibit antagonistic activity on cells stimulated with human IL-6 (data not shown). Such assays have to be performed at 37 °C a temperature at which D3 is already unfolded. Since a recombinant version of sIL-6R consisting of D2 and D3 is stable at 37 °C (20), it can be concluded that in this complex D2 and D3 must stabilize each other.
It has been suggested recently that the complex of IL-6, IL-6R, and gp130 has a stochiometry of two molecules each of IL-6, IL-6R, and gp130 (41-43). Steric considerations led us to suggest a tetrameric model of the receptor complex containing one molecule each of IL-6 and IL-6R associated with two molecules of gp130 (36). Of note, our tetrameric model would predict a close contact of D2 of IL-6R with one gp130 protein (36). In this respect it is worth mentioning that mutation of valine 190 in the human IL-6R resulted in loss of complex formation between IL-6·IL-6R and gp130 (19), whereas IL-6 binding to IL-6R was unchanged (19). Valine 190 resides within D2 (22). A peptide corresponding to a part of D3 in the human IL-6R was shown to inhibit the biological activity of IL-6 without disturbing binding of IL-6 to IL-6R (44). From these data it can be concluded that both D2 and D3 seem to be involved in complex formation between IL-6·IL-6R and gp130.
Our data add to the understanding of the molecular mechanism of the association of the components IL-6, IL-6R, and gp130 in the receptor complex. Futhermore no experimental structural information is available on human IL-6R, the reported strategy of bacterial expression and refolding of the IL-6R domain, which is important for ligand binding, might be the basis for experiments aiming at structure elucidation by NMR spectroscopy or x-ray crystallography.
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FOOTNOTES |
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* This work was supported by grants from the Deutsche Forschungsgemeinschaft (Bonn, Germany) and the Stiftung Rheinland-Pfalz für Innovation (Mainz, Germany).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.
§ To whom correspondence should be addressed: I. Medizinische Klinik, Abteilung Pathophysiologie, Johannes Gutenberg-Universität Mainz, Obere Zahlbacher Str. 63, D-55101 Mainz, Germany. Tel.: 49-6131-173363; Fax: 49-6131-173364; E-mail: rosejohn{at}mail.uni-mainz.de.
The abbreviations used are: IL, interleukin; CT-1, cardiotrophin-1; CTNF, ciliary neurotrophic factor; LIF, leukemia inhibitory factor; OSM, oncostatin M; CBM, cytokine-binding module; PCR, polymerase chain reaction; PAGE, polyacrylamide gel electrophoresis; ELISA, enzyme-linked immunosorbent assay; PBS, phosphate-buffered saline; POD, peroxidase.
2 T. Jostock, S. Rose-John, and J. Müllberg, manuscript in preparation.
3 P. Vollmer, B. Oppmann, N. Voltz, and S. Rose-John, submitted for publication.
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REFERENCES |
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