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Originally published In Press as doi:10.1074/jbc.M102293200 on November 8, 2001
J. Biol. Chem., Vol. 277, Issue 4, 2511-2516, January 25, 2002
The  -Chains of C4b-binding Protein Mediate Complex Formation
with Low Density Lipoprotein Receptor-related Protein*
Erik
Westein ,
Cécile V.
Denis§,
Bonno N.
Bouma, and
Peter J.
Lenting¶
From the Laboratory for Thrombosis and Haemostasis,
Department of Haematology, University Medical Center Utrecht, 3584 CX
Utrecht, The Netherlands and § INSERM U143, Hôpital
Bicêtre, 94276 le Kremlin-Bicêtre, France
Received for publication, March 14, 2001, and in revised form, October 11, 2001
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ABSTRACT |
C4b-binding protein (C4BP) is a
heparin-binding protein that participates in both the complement and
hemostatic system. We investigated the interaction between C4BP and low
density lipoprotein receptor-related protein (LRP), an endocytic
receptor involved in the catabolism of various heparin-binding
proteins. Both plasma-derived C4BP and recombinant C4BP consisting of
only its  -chains (rC4BP) bound efficiently to immobilized LRP, as
determined by surface plasmon resonance analysis. Complementary, two
distinct fragments of LRP, i.e. clusters II and IV, both
associated to immobilized rC4BP, and binding could be inhibited by
the LRP antagonist receptor-associated protein. Further analysis showed
that association of rC4BP to LRP was inhibited by heparin or by
anti-C4BP antibody RU-3B9, which recognizes the heparin-binding region
of the C4BP -chains. In cellular degradation experiments,
LRP-expressing fibroblasts effectively degraded
125I-labeled rC4BP, whereas their LRP-deficient
counterparts displayed a 4-fold diminished capacity of degrading
125I-rC4BP. Finally, initial clearance of C4BP in mice
was significantly delayed upon co-injection with receptor-associated
protein. In conclusion, our data demonstrate that the -chains of
C4BP comprise a binding site for LRP. We propose that LRP mediates at
least in part the catabolism of C4BP and, as such, may regulate
C4BP participation in complement and hemostatic processes.
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INTRODUCTION |
C4b-binding protein
(C4BP)1 is a plasma protein,
which serves as a regulator of the complement system (1). C4BP
binds the complement protein C4b, which results in enhancement
of factor I-mediated degradation of C4b and inhibition of the classical pathway C3 convertase (C4b2a) complex (1). In plasma, C4BP may serve as
a carrier protein for at least two other plasma proteins: the vitamin
K-dependent anticoagulant Protein S and serum amyloid P
component (1). In addition, C4BP may interact with coagulation factor
VIII as well (2). The majority of the C4BP molecules (~80%) consist
of seven identical -chains and a unique  -chain, whereas other
isoforms lack either one of the -chains or the -chain (3). The
-chain is involved in the interaction with Protein S (4), and
complex formation with serum amyloid P component (SAP) and complement
proteins is mediated by the -chains (5, 6). In addition, the
-chains have been found to contain binding sites for bacterial
surface proteins from Streptococcus pyogenes (7) and heparin
(8). The heparin interactive site, which overlaps with the C4b
interactive site, encompasses a cluster of positively charged amino
acids involving Arg residues at positions 39, 64, and 66 (9).
The average plasma concentration of C4BP is ~260 nM (150 µg/ml) (10), although its levels may increase up to 4-fold during inflammation, infection, or tissue damage (11, 12). Plasma levels
represent a balance between C4BP production and removal. At present,
little is known concerning the molecular mechanisms that control the
removal of C4BP from the circulation. The notion that C4BP is able to
interact with heparin opens the possibility that C4BP may interact with
heparan sulfate proteoglycans (HSPG) exposed at the cellular surface.
Alternatively, C4BP may interact with cellular receptors like the low
density lipoprotein receptor-related protein (LRP), which is known to
recognize heparin-binding proteins.
LRP, also known as the 2-macroglobulin receptor, is a
member of the low density lipoprotein receptor family of endocytic receptors (13, 14). It consists of a noncovalently linked heavy and
light chain. The 85-kDa light chain comprises the transmembrane and
cytoplasmic domains, whereas the ligand binding regions are located
within the 515-kDa heavy chain (15). The heavy chain contains four
domains enriched in low density lipoprotein receptor class A domains,
generally referred to as clusters I-IV. It has been reported that
clusters II and IV play a prominent role in ligand binding to the
receptor (16).
LRP is widely distributed among tissues, such as liver, brain, and
placenta, and is expressed in an array of cell types including parenchymal cells, Kupffer cells, neurons, astrocytes, smooth muscle
cells, monocytes, and fibroblasts (17). LRP has traditionally been
reported as a receptor that is involved in hepatic clearance of
numerous proteins (18), although recent studies demonstrate that LRP
contributes to cellular signaling processes as well (19). Ligands bound
by LRP belong to a spectrum of structurally and functionally unrelated
proteins (13, 14, 18). These include apolipoproteins, lipases,
proteinases, proteinase/inhibitor complexes, Kunitz-type inhibitors,
matrix proteins, and several others.
The mechanism by which binding to LRP is mediated varies between
ligands. First, ligands (e.g.
2-macroglobulin/protease complexes) may bind directly
from the circulation to LRP (20, 21). Alternatively, binding may be
promoted by so called accessory proteins. This possibility is
exemplified by the urokinase-type plasminogen activator receptor, which
facilitates internalization of urokinase complexed with its inhibitor
plasminogen activator inhibitor-1 by LRP (22, 23). Furthermore,
LRP-mediated degradation may be preceded by sequestration of the
ligands by HSPG. Examples hereof include -amyloid precursor protein
(24), tissue factor pathway inhibitor (25), activated factor IX (26),
and thrombospondin (27).
In the present study, we assessed binding of C4BP to LRP by surface
plasmon resonance (SPR) employing purified components. Our data show
that C4BP is able to interact with LRP with moderate affinity, and that
binding involves the C4BP -chain and the cluster II and IV regions
of LRP. Furthermore, we found that LRP mediates the delivery of
rC4BP to the intracellular degradation pathway in mouse fibroblast
cells, and that the initial clearance of C4BP in mice is delayed upon
co-injection with the LRP-antagonist receptor-associated protein. Our
data suggest that LRP contributes to the catabolism of the complement
protein C4BP.
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EXPERIMENTAL PROCEDURES |
Materials--
The Biacore2000 biosensor system and reagents,
including an amine-coupling kit and CM5 biosensor chips (research
grade), were from Biacore AB (Uppsala, Sweden). Cell culture plates,
Dulbecco's modified Eagle's medium (DMEM), DMEM/F-12 medium, fetal
calf serum, penicillin, and streptomycin were from
Invitrogen (Breda, The Netherlands). Unfractionated heparin was
purchased from Sigma (Zwijndrecht, The Netherlands). Protein
G-Sepharose was from Amersham Biosciences, Inc.
Proteins--
Plasma-derived C4BP (pd-C4BP) and Protein S were
purified as described (28, 29). Recombinant C4BP, consisting of the
-chains but lacking the -chain (rC4BP), was produced using
stably transfected baby hamster kidney cell lines, purified until
homogeneity by immunoaffinity chromatography as reported previously
(30), and stored in 125 mM NaCl, 0.005% (v/v) Tween 20, 25 mM Hepes (pH 7.4) at  20 °C. Purified rC4BP was
labeled with Na125I (Amersham Biosciences, Inc.) using the
IODO-GEN method (Pierce) as described (8). Free Na125I was
removed by chromatography on a PD-10 column (Amersham Biosciences, Inc.) equilibrated in 125 mM NaCl, 0.005% (v/v) Tween 20, 25 mM Hepes (pH 7.4), and 125I-labeled rC4BP
was stored in small aliquots at 20 °C. Specific radioactivity was
4.0 (± 1.3) × 105 cpm/pmol rC4BP (mean ± S.E.; n = 6). Each radiolabeled rC4BP preparation
was compared with unlabeled rC4BP for binding to immobilized LRP
employing SPR. In all cases labeled and unlabeled preparations
displayed similar sensorgrams, demonstrating that both association and
dissociation characteristics were unchanged upon labeling. On one
occasion, this was investigated in more detail by determining affinity
constants, which proved to be similar for radiolabeled and unlabeled
rC4BP (3.5 and 55.2 nM versus 5.6 and 66.2 nM, respectively). Purified full-length LRP (31) was kindly
provided by Dr. S. K. Moestrup (University of Aarhus, Aarhus,
Denmark). Receptor-associated protein fused to glutathione S-transferase (GST-RAP) (32) was prepared as described
previously (33). Recombinant LRP fragments encompassing LRP cluster II and cluster IV were produced using stably transfected baby hamster kidney cell lines, which were kindly provided by Dr. H. Pannekoek (University of Amsterdam, Amsterdam, The Netherlands). Clusters were purified employing GST-RAP affinity chromatography as described (16) and stored at 4 °C in 125 mM NaCl, 1 mM
CaCl2, 0.005% (v/v) Tween 20, 25 mM Hepes (pH
7.4). Monoclonal antibody RU-3B9 (34) was purified from ascites using
protein G-Sepharose as recommended by the manufacturer. RU-3B9 Fab
fragments were prepared using the ImmunoPure Fab preparation kit
(Pierce) as instructed. Bovine serum albumin (fraction V) was obtained
from Sigma. Proteins were quantified by a BCA protein assay (Pierce)
using albumin as a standard.
SPR Analysis--
Binding studies were performed
employing a Biacore2000 biosensor system, and SPR analysis was done
essentially as described (26, 33). LRP or rC4BP was immobilized on a
CM5 sensor chip at the indicated densities using the amine-coupling kit
as instructed by the supplier. Routinely, a control channel was
activated and blocked using the amine-coupling reagents in the absence
of protein. Binding to coated channels was corrected for binding to
noncoated channels (<5% of binding to coated channels). SPR analysis
was performed in 125 mM NaCl, 0.005% (v/v) Tween 20, 25 mM Hepes (pH 7.4) at 25 °C at indicated flow rates.
Regeneration of the surface of the LRP sensor chip was performed by
subsequent application of 100 mM
H3PO4 and 25 mM CaCl2.
The rC4BP sensor chip was regenerated using 100 mM
H3PO4.
Analysis of Quantitative SPR Data--
For analysis of
association and dissociation curves of the sensorgrams, BiaEvaluation
software was used (Biacore AB). Interaction constants were determined
by performing nonlinear global fitting of data corrected for bulk
refractive index changes. Data were fitted to various models available
within the software. For binding of rC4BP to immobilized LRP, a
model describing the interaction between rC4BP and two independent
binding sites (heterologous ligand, parallel reactions) was found to
provide the best fit of the experimental data. Accuracy of the fits was
judged from residual plots and statistical parameters employing
previously described equations (35).
Statistical Analysis--
Statistical significance of clearance
data (see Fig. 4) and of association and dissociation rate constants
(see Table I) were calculated using Student's unpaired t
test employing the InStat program (GraphPad Software, Inc.).
Cellular Degradation Experiments--
Cellular degradation of
rC4BP was examined using mouse fibroblast cell lines MEF-1 (American
Tissue Culture Collection, CRL-2214), or their counterparts, which are
genetically deficient for LRP, PEA-13 (American Tissue Culture
Collection, CRL-2216). MEF-1 and PEA-13 cells have been isolated from
embryos resulting from the mating of mice heterogenous for LRP gene
disruption (36). The MEF-1 cells express LRP endogenously, whereas
PEA-13 cells have been demonstrated to contain two (via homologous
recombination) disrupted alleles for the LRP gene. Cells were seeded at
least 48 h before the experiment and grown to 90-95% confluence
in 24-well plates in DMEM supplemented with 10% (v/v) fetal calf
serum, 100 units/ml penicillin, and 100 µg/ml streptomycin. Before
incubation, cells were extensively washed with DMEM/F-12 medium.
125I-labeled rC4BP was mixed with nonlabeled rC4BP to
a 1:1 molar ratio, and the mixture was then added to the cells in a
final volume of 250 µl in incubation medium (DMEM/F-12 medium
supplemented with 1% (w/v) bovine serum albumin and 2 mM
CaCl2). Final concentration of rC4BP was 100 nM. After a 1-h incubation at 4 °C, cells were washed
three times with 500 µl of incubation medium to remove nonbound
material. Subsequently, incubation was allowed to proceed at 37 °C
in a volume of 250 µl. At indicated time points, samples were taken
to determine the amount of degraded material. Degraded material is
defined as the radioactivity that is soluble in 10% trichloroacetic
acid. In all experiments a control was included in which the amount of
degradation was examined in the absence of cells.
Clearance of Human C4BP in C57BL/6J Mice--
We used
14-16-week- old C57BL/6J mice. Three to six mice were housed in each
cage and fed a standard chow diet and water ad libitum. Mice
were injected intravenously with pd-C4BP (10.9 mg/kg) alone or in
combination with GST-RAP (30 mg/kg) into the tail vein. Blood samples
were collected in polypropylene Eppendorf tubes, containing
approximately 0.1 volume of 129 mM trisodium citrate, at
indicated time points from anesthetized mice by retro-orbital venous
plexus puncture. Plasma was prepared by centrifugation of the blood at
2500 × g for 20 min at room temperature. Residual C4BP
was determined using an immunosorbent assay specific for human C4BP.
For each time point, 3 mice were used.
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RESULTS |
C4BP Binding to Immobilized LRP--
Binding of pd-C4BP to LRP was
investigated by SPR analysis using purified components. An increase in
response was observed when pd-C4BP (30 nM) was passed over
immobilized LRP (7 and 11 fmol/mm2), demonstrating that
pd-C4BP is able to associate with LRP (Fig. 1A). As the highest response
is observed at the highest density of LRP, binding appears to be
dose-dependent. Replacement of pd-C4BP solution by buffer
resulted in a gradual decline of the response, indicating that pd-C4BP
dissociates from LRP and that binding is reversible (Fig.
1A). In plasma, C4BP is able to associate with other plasma
proteins, like Protein S and SAP. Our data therefore do not fully
exclude that the observed response originates from traces of Protein S
or SAP present within the pd-C4BP preparation. However, no additional
response was observed upon subsequent injection of anti-Protein S or
anti-SAP antibodies after injection of C4BP preparations (data not
shown). In addition, no association of purified Protein S to
immobilized LRP was detected (Fig. 1A). Apparently, the
observed increase in response originates from binding of C4BP to
LRP.
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Fig. 1.
Binding of plasma-derived and recombinant
C4BP to immobilized LRP. A, LRP immobilized at a CM5
sensor chip at a density of 7 or 11 fmol/mm2
(lines II and I, respectively) was
incubated with pd-C4BP (30 nM) in 125 mM NaCl,
0.005% (v/v) Tween 20, and 25 mM Hepes (pH 7.4) at a flow
rate of 5 µl/min for 2 min at 25 °C. Ligand solution was replaced
with buffer to initiate dissociation. Line III
represents incubation of immobilized LRP (11 fmol/mm2) with
Protein S (400 nM) under similar conditions. B,
seven different concentrations (2, 4, 7, 10, 15, 20, and 30 nM) of rC4BP were passed over immobilized LRP (11 fmol/mm2) at 25 °C for 3 min at a flow rate of 20 µl/min. The subsequent association and dissociation of rC4BP is
represented by the seven data curves
shown. Lines represent the data curves and their fitted
curves obtained using a model for heterologous ligand (parallel
reaction) interactions. For both graphs, the signal is indicated in
resonance units (RU) and is corrected for aspecific binding,
which was less than 5% of binding to LRP-coated channels.
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LRP Binding Involves -Chains of C4BP--
To further
characterize the interaction between C4BP and LRP, SPR analysis was
performed employing purified recombinant C4BP that consists only of the
-chains (30). As shown in Fig. 1B, recombinant rC4BP
(2-30 nM) efficiently associated to immobilized LRP (11 fmol/mm2) in a dose-dependent manner. Binding
appeared to be similar for plasma-derived and recombinant C4BP. The
interaction between rC4BP and immobilized LRP was studied in more
detail by assessment of the apparent association and dissociation rate
constants, which are summarized in Table
I. Experimental data were fitted most appropriately using a model describing the interaction of rC4BP with
two classes of binding sites (heterologous ligand, parallel interactions). The resulting apparent affinity constants
(Kd(app)) values were 2.4 ± 1.9 nM and 71.4 ± 42.5 nM, respectively.
These data demonstrate that LRP is able to bind the C4BP -chain with moderate affinity in a reversible and dose-dependent
manner.
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Table I
Kinetic parameters for the binding of rC4BP to LRP
Association and dissociation of various concentrations rC4BP to LRP
(11 fmol/mm2) was assessed as described in the legend of Fig.
1. Buffer consisted of 0.005% (v/v) Tween 20, 25 mM Hepes
(pH 7.4) supplemented with either 50 or 125 mM NaCl.
rC4BP concentrations tested varied between 2 and 30 nM.
The data obtained for all concentrations tested were analyzed to
calculate apparent association rate constants
(kon(app)) and apparent dissociation rate constants
(koff(app)) as described using a two-site binding
model (35). Each class of binding sites is referred to as 1 and 2, respectively. Apparent affinity constants
(Kd(app)) were inferred from the ratio
koff(app):kon(app). Data are
based on three to six measurements using four or five different
concentrations for each measurement. Data represent the average (± S.D.). p values were calculated employing Student's
unpaired t test.
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Binding of Recombinant LRP Fragments to Immobilized
rC4BP--
The observation that C4BP interacts with two different
binding sites may suggest heterogeneity of LRP because of its
immobilization. Alternatively, LRP may comprise distinct regions that
are able to interact with C4BP -chains. To identify LRP regions
involved in binding C4BP -chains, purified recombinant receptor
fragments were used. These fragments, designated cluster II and IV,
respectively, have been established to encompass the ligand binding
domains of LRP (16). When either cluster (200 nM) was
incubated with immobilized recombinant rC4BP (10 fmol/mm2), reversible binding of cluster II and IV to
rC4BP was observed (Fig.
2A). The specificity of the
interaction was subsequently assessed by investigating the binding of
cluster II or IV to immobilized rC4BP in the presence of various
concentrations of the LRP-antagonist GST-RAP. Indeed, GST-RAP (0-750
nM) efficiently interfered with binding of either cluster
(150 nM) to immobilized rC4BP (Fig. 2B).
Thus, both recombinant LRP fragments encompassing the ligand binding
domains, i.e. clusters II and IV, comprise a binding site for rC4BP, and binding is inhibited in the presence of GST-RAP.
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Fig. 2.
SPR analysis of the interaction between
rC4BP and recombinant LRP fragments.
A, rC4BP immobilized at a CM5 sensor chip at a density of
10 fmol/mm2 was incubated with 185 nM LRP
cluster II (line I) or LRP cluster IV
(line II) as described in the legend of Fig.
1A. B, binding of 150 nM cluster II
(open squares) or cluster IV (closed
squares) to immobilized rC4BP (10 fmol/mm2)
was analyzed by SPR (flow rate 10 µl/min) in the absence or presence
of GST-RAP (0-750 nM). Binding is expressed as percentage
of maximal response in the absence of GST-RAP and is corrected for
nonspecific binding (<5%). Data represent the mean ± S.D. of
three experiments.
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Cellular Degradation of 125I-rC4BP Is Mediated by
LRP--
The observation that LRP recognizes C4BP in a system
employing purified components prompted us to investigate the
contribution of LRP to the delivery of rC4BP to the intracellular
degradation pathway. This was addressed in experiments using mouse
fibroblast cells genetically deficient for LRP (i.e. PEA-13
cells), or their counterparts expressing LRP endogenously
(i.e. MEF-1 cells) (36). Employing LRP-expressing MEF-1
cells, an increase in the amount of degraded 125I-labeled
rC4BP was observed in time (Fig. 3).
However, when degradation was examined in the presence of 1 µM GST-RAP, the amount of 125I-labeled
rC4BP degraded was markedly reduced (Fig. 3), indicating that the
degradation process involves a GST-RAP-sensitive receptor. In the
presence of LRP-deficient PEA-13 cells, the amount of rC4BP degraded
was similar to that of MEF-1 cells in the presence of the LRP
antagonist GST-RAP (Fig. 3). Together, these data strongly suggest that
the cellular uptake and transport of 125I-rC4BP to the
intracellular degradation pathway involves a LRP-dependent pathway.
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Fig. 3.
Cellular degradation of
125I-labeled rC4BP. MEF-1
cells either in the presence (open squares) or
absence of GST-RAP (closed squares) or PEA-13
cells (closed circles) were incubated with a 1:1
mixture of unlabeled and 125I-labeled rC4BP (final
concentration 100 nM) at 4 °C for 60 min. After washing,
bound material was subsequently incubated at 37 °C for indicated
time points, and degradation of rC4BP was determined as described
under "Experimental Procedures." Data represent the mean ± S.E. of four to six experiments.
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In Vivo Clearance of Human pd-C4BP Is Modulated by GST-RAP--
To
investigate whether LRP also contributes to the clearance of C4BP
in vivo, human pd-C4BP (10.9 mg/kg) was injected
intravenously into the tail vein of C57BL/6J mice in the absence or
presence of GST-RAP (30 mg/kg). At indicated time points, blood samples were collected, and plasma was subsequently analyzed for residual C4BP
content. As shown in Fig. 4, human
pd-C4BP was cleared in mice in a biphasic manner with an initial
half-life of ~50 min, whereas, in the presence of GST-RAP, pd-C4BP
was cleared at a slower rate (approximate half-life of 60 min). At the
15- and 30-min time points, the content of C4BP was significantly
higher (p = 0.0026 and p = 0.0098, respectively) in the presence of GST-RAP than in the absence of this
LRP-antagonist. Apparently, inhibition of GST-RAP-sensitive receptors,
like LRP, is associated with a delay in initial clearance of C4BP.
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Fig. 4.
In vivo clearance of human pd-C4BP
in mice. Mice were injected with human pd-C4BP (10.9 mg/kg) in the
absence (open circles) or presence
(closed circles) of GST-RAP (30 mg/kg). At
indicated time points, blood samples were taken and plasma was examined
for pd-C4BP content employing an immunosorbent assay specific for human
C4BP. Each data point represents the average (± S.D.) of three
individual mice. The amount of pd-C4BP detected at time points 15 and
30 min, is significantly higher in the presence than in the absence of
GST-RAP (p = 0.0026 and p = 0.0098, respectively).
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Interaction between rC4BP and LRP Is Ionic
Strength-dependent--
It has been reported that binding
of the C4BP -chains to C4b is strongly ionic
strength-dependent, whereas binding of streptococcal M
proteins to these -chains is of more hydrophobic nature (9). To
investigate the nature of the -chain/LRP interaction, association of
rC4BP (20 nM) to immobilized LRP (11 fmol/mm2) was examined in 0.005% (v/v) Tween 20, 25 mM Hepes (pH 7.4), supplemented with various concentrations
of NaCl (25-150 mM). As shown in Fig.
5, association of rC4BP to LRP was
sensitive to the concentration of NaCl. Optimal association was
observed at 35 mM NaCl, whereas association was reduced
over 6-fold at NaCl concentrations exceeding 100 mM. To
further examine the effect of NaCl on the rC4BP/LRP
interaction, the apparent association and dissociation rate constants
were determined employing 50 mM NaCl. As for the assessment
of the rate constants in the presence of 125 mM NaCl,
binding of rC4BP to LRP involved two classes of binding sites (Table
I). With regard to the calculated rate constants, no significant
differences were found, except for the class 2 association rate
constant. Class 2 kon(app) determined at 50 mM NaCl proved to differ significantly from class 2 kon(app) determined at 125 mM NaCl
(p = 0.024). A 4-fold increase in association rate
constant at 50 mM NaCl resulted in a subsequent 4-fold
higher affinity of rC4BP for immobilized LRP.
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Fig. 5.
Effect of NaCl concentration on
rC4BP/LRP interaction. rC4BP (20 nM) was incubated with immobilized LRP (11 fmol/mm2) in a buffer containing 0.005% (v/v) Tween 20, 25 mM Hepes (pH 7.4), and varying concentrations of NaCl
(25-150 mM) at 25 °C using a flow rate of 20 µl/min.
Association was allowed to proceed for 2 min, and the response
(RU) after 2 min of association is indicated.
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Inhibition of rC4BP/LRP Interaction by Monoclonal Antibody
RU-3B9--
The observation that the rC4BP/LRP interaction displays
a sensitivity to NaCl similar to that described for the C4b/C4BP interaction (Fig. 5; Ref. 9) may suggest that C4b and LRP bind to a
similar region within the -chains of C4BP. Previously, monoclonal antibody RU-3B9, which is directed against C4BP, has been shown to
interfere with the binding of C4b to C4BP. Therefore, the effect of Fab
fragments of this antibody (0-320 nM) on the binding of rC4BP (40 nM) to immobilized LRP (11 fmol/mm2) was tested by SPR-analysis. Fab RU-3B9 indeed
inhibited binding of rC4BP to immobilized LRP, and binding was fully
suppressed at 80 nM RU-3B9 (Fig.
6A). Inhibition appeared to be
specific because Fab RU-3B9 was unable to affect binding of another LRP ligand (factor VIII light chain; Ref. 33) to LRP (data not shown). These data indicate that the LRP binding site may overlap with the
RU-3B9 binding site within the C4BP -chain.
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Fig. 6.
Effect of antibody RU-3B9 and heparin on the
rC4BP/LRP interaction. 40 nM
of rC4BP was allowed to associate for 2 min to immobilized LRP (11 fmol/mm2) in the absence or presence of various
concentrations of Fab RU-3B9 (panel A) or heparin
(panel B) in 125 mM NaCl, 0.005% (v/v) Tween
20, 25 mM Hepes (pH 7.4) at 25 °C at a flow rate of 10 µl/min. Binding is expressed as the percentage of binding in the
absence of competitor and is corrected for nonspecific binding (<5%).
Data are mean ± S.D. of three experiments. Inset,
degradation of 125I-labeled rC4BP by MEF-1 cells was
assessed as described in the legend of Fig. 3, in the absence
(closed squares) or presence (open
squares) of 750 nM Fab RU-3B9 (panel
A) or 0.25 mg/ml heparin (panel B).
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Binding of rC4BP to LRP Is Inhibited in the Presence of
Heparin--
It has been reported previously that the
-chain-directed antibody RU-3B9 prevents binding of C4BP to heparin
(8). It was of interest, therefore, to examine the effect of heparin on
binding of rC4BP to LRP. As expected, normal binding was detected in the absence of heparin as assessed by SPR analysis (Fig.
6B). In the presence of increasing concentrations of
heparin, however, a decrease of the resonance signal was observed.
Half-maximal inhibition was obtained at 0.2 mg/ml heparin. We
anticipated that, if binding of rC4BP to LRP was inhibited by
heparin or RU-3B9 in a system employing purified components, both
components should also interfere with the intracellular degradation of
rC4BP by LRP-expressing cells. Indeed, the amount of
125I-labeled rC4BP by LRP-expressing MEF-1 cells was
reduced 4- and 3-fold in the presence of RU-3B9 and heparin,
respectively (Fig. 5, A and B,
insets). Our data seem to be compatible with a model in
which the heparin-binding region within the C4BP -chains overlaps
with an interactive site for LRP.
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DISCUSSION |
A first step in resolving the pathways that mediate the clearance
of proteins is the identification of cellular receptors that control
the endocytosis of the protein of interest. In the present study, we
provide evidence that the endocytic pathway of the complement
regulatory protein C4BP involves LRP, a hepatic receptor established to
be responsible for the clearance of various other plasma proteins (14,
18). First, in a system employing purified components, C4BP and a
recombinant derivative thereof (rC4BP) both associated to
immobilized LRP in a reversible and dose-dependent manner
(Fig. 1). In complementary experiments, we show that soluble,
recombinant fragments of LRP associate to immobilized rC4BP and that
this association is inhibited in the presence of GST-RAP, an antagonist
of ligands binding to LRP (Fig. 2). Further, LRP-deficient mouse
fibroblasts display diminished capacity compared with LRP-expressing
fibroblasts in degrading rC4BP, and cellular degradation of rC4BP
by LRP-expressing cells was markedly reduced in the presence of the
LRP-antagonist GST-RAP (Fig. 3). Finally, in the presence of GST-RAP,
the initial clearance of C4BP was significantly delayed
(Fig. 4). C4BP is the third component of the complement pathway that
has been reported to be a ligand for LRP. Storm and co-workers (37)
reported that C1 inhibitor/C1s complexes are cleared from the
circulation in a process that involves LRP. In addition, Meilinger
et al. (38) showed that the catabolism of the activated
complement component C3 is mediated by LRP. C4BP, however, seems to be
different from both these ligands in its interaction with LRP. Whereas
C1 inhibitor/C1s and C3 are recognized by LRP after complex formation
and proteolysis, respectively, C4BP is recognized by LRP in its native
circulating form. As such, C4BP is the first identified member of the
complement protein family whose plasma levels and function may be
directly regulated by LRP.
Analysis of the SPR data suggested that the interaction between
rC4BP and immobilized LRP could be described employing a two-site
binding model (Table I). The presence of multiple binding sites within
LRP may result from heterogeneity of LRP because of its immobilization
onto the biosensor chip. Alternatively, LRP may comprise multiple
regions, which are able to interact with rC4BP. Indeed, recombinant
fragments of LRP comprising distinct regions of the LRP molecule
(i.e. clusters II and IV, respectively) proved able to
associate with rC4BP (Fig. 2A). Noteworthy, the apparent
Kd values for assembly of the C4BP/LRP complex (i.e. 2.4 and 71.4 nM, Table I) are well below
the plasma levels of C4BP (260 nM; Ref. 10). This would
allow a continuous formation of the C4BP/LRP complex in vivo
and subsequent removal of C4BP from the circulation. It should be
mentioned, however, that, to calculate the apparent rate constants,
molar concentrations of C4BP based on protein levels were used. Because
each molecule contains seven identical -chains (1), the actual
number of potential binding sites is 7-fold the molar C4BP
concentration. For binding of C4b protein to C4BP, it has been reported
that, after four molecules of C4b have bound to C4BP, the binding of additional C4b molecules is sterically hindered (39). In view of this
observation, it seems likely that only part of the seven potential
binding sites are available for complex formation between C4BP and LRP.
In our opinion, it is therefore reasonable to assume that the actual
affinities are severalfold less stringent compared with the affinities
that are summarized in Table I. The in vivo survival
experiments, however, have been performed employing C4BP plasma levels
of 190 nM, which is ~25% below the levels reported for
human plasma. Nevertheless, C4BP was rapidly cleared (Fig. 4),
indicating that physiological conditions allow complex formation between C4BP and LRP. It should be mentioned, however, that the clearance experiments do not completely rule out the possibility that
other receptors contribute to C4BP clearance as well. First, GST-RAP is
not a selective inhibitor of LRP, but recognizes also other members of
the low density lipoprotein family, like megalin or apolipoprotein E
receptor 2. Second, the notion that C4BP comprises a binding site for
heparin suggests that also HSPG may be involved in the cellular uptake
of C4BP. Whether this proceeds via direct internalization of C4BP by
HSPG or via HSPG-mediated sequestration at the cellular surface before
delivery to LRP is currently under investigation.
Complement protein C4b and heparin have been reported to share
overlapping binding sites within a region located at the interface between the so called complement control protein domains 1 and 2 of the
C4BP -chains (9, 40). This region is particularly enriched in
positively charged amino acids, and residues Arg-39, Lys-63, and Arg-64
appear to be especially critical for C4b and heparin binding.
Apparently, binding of these components to C4BP is mainly mediated by
electrostatic interactions, which is supported by the observation that
complex formation between C4BP and C4b or heparin is sensitive to NaCl
(9, 40). The interaction between rC4BP and LRP displayed a
strikingly similar NaCl dependence as described for the C4b/C4BP and
heparin/C4BP interactions (Fig. 5; Refs. 9 and 40). Further, binding of
rC4BP to LRP was inhibited effectively by heparin, as well as by an
antibody known to inhibit binding of C4BP to both heparin and C4b (Fig.
6). With regard to these observations, it seems conceivable that a LRP interactive site is similar or close to the reported binding site for
C4b within the -chains of C4BP. As such, LRP may interfere with
C4BP-dependent down-regulation of C4b and the C3 convertase complex.
Apart from its role in the complement system, C4BP is functionally
related to the hemostatic system as well. In plasma, C4BP may serve as
a carrier protein for the anticoagulant component Protein S, and
~60% of the Protein S molecules are noncovalently bound to C4BP
(41). When bound to the -chain of C4BP, Protein S is unable to exert
its cofactor activity to the Protein C anticoagulant pathway (42),
indicating that C4BP contributes to the regulation of Protein S
cofactor activity. Although speculative, our finding that the
catabolism of C4BP could involve a LRP-dependent process may imply that LRP indirectly affects catabolism of Protein S as well.
This would provide an extra link between the hemostatic process and
LRP. Previously, it has been reported that LRP contributes to the
clearance of thrombin/antithrombin and factor
Xa/2-macroglobulin complexes (43, 44), and the cellular
uptake of coagulation proteins factor VIII (33, 45) and activated
factor IX (26). In addition, LRP contributes to the tissue factor
pathway inhibitor-dependent down-regulation of tissue
factor/factor VIIa complex at the surface of monocytes and fibroblasts
(46, 47). The notion that LRP is involved in the cellular uptake of
both pro- and anticoagulant proteins may indicate that LRP serves a so
far unrecognized role in the regulation of the coagulation process.
| |
FOOTNOTES |
*
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: Dept. of
Haematology, University Medical Center Utrecht, Heidelberglaan 100, 3584 CX Utrecht, The Netherlands. Tel.: 31-30-250-7610; Fax:
31-30-251-1893; E-mail: p.j.lenting@lab.azu.nl.
Published, JBC Papers in Press, November 8, 2001, DOI 10.1074/jbc.M102293200
| |
ABBREVIATIONS |
The abbreviations used are:
C4BP, C4b-binding
protein;
pd-C4BP, plasma-derived C4b-binding protein;
rC4BP, recombinant C4b-binding protein consisting of only its -chains;
DMEM, Dulbecco's modified Eagle's medium;
GST-RAP, receptor-associated protein fused to glutathione
S-transferase;
LRP, low density lipoprotein receptor-related
protein;
SPR, surface plasmon resonance;
HSPG, heparan sulfate
proteoglycan;
SAP, serum amyloid P component.
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ABSTRACT
INTRODUCTION