Vol. 283, Issue 2, R339-R346, August 2002
Loss of albumin and megalin binding to renal cubilin in rats
results in albuminuria after total body irradiation
Raghunatha R.
Yammani1,2,
Mukut
Sharma3,
Shakuntla
Seetharam1,2,
John E.
Moulder4,
Nancy M.
Dahms5, and
Bellur
Seetharam1,2,5
1 Department of Medicine, Divisions of
2 Gastroenterology and Hepatology and 3 Nephrology;
and Departments of 4 Radiation Oncology and
5 Biochemistry, Medical College of Wisconsin and
Veterans Affairs Medical Center, Milwaukee, Wisconsin 53226
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ABSTRACT |
The role of the
renal apical brush-border membrane (BBM) endocytic receptors cubilin
and megalin in the onset of albuminuria in rats exposed to a
single dose of total body irradiation (TBI) has been investigated.
Albuminuria was evident as immunoblot (IB) analysis of the urine
samples from TBI rats revealed excretion of large amounts of albumin.
IB analysis of the BBM proteins did not reveal any significant changes
in cubilin or megalin levels, but 125I-albumin binding to
BBM from TBI rats declined by 80% with a fivefold decrease (from 0.5 to 2.5 µM) in the affinity for albumin. IB analysis of cubilin from
the BBM demonstrated a 75% loss when purified using albumin, but not
intrinsic factor (IF)-cobalamin (Cbl) ligand affinity chromatography.
Immunoprecipitation (IP) of Triton X-100 extract of the BBM with
antiserum to cubilin followed by IB of the immune complex with an
antiserum to megalin revealed a 75% loss of association between
megalin and cubilin. IP studies with antiserum to cubilin or megalin
and IB with antiserum to the cation-independent mannose
6-phosphate/insulin-like growth factor II-receptor (CIMPR) revealed
that CIMPR interacted with both cubilin and megalin. In addition, TBI
did not disrupt the association of CIMPR with either cubilin or megalin
in BBM. These results suggest that albuminuria noted in TBI rats is due
to selective loss of albumin and megalin, but not CIMPR or IF-Cbl
binding by cubilin. Furthermore, these results also suggest
that albumin and IF-Cbl binding to cubilin occur at distinct sites and
that in the rat renal BBM, CIMPR interacts with both cubilin and megalin.
endocytic receptors; endocytosis
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INTRODUCTION |
CUBILIN is a
460-kDa multidomain (24) cell surface glycoprotein
receptor that is expressed in the intestine, kidney, and yolk sac
(31). In the intestine it plays an important role in the
uptake of dietary cobalamin (Cbl; vitamin B12), while in
the kidney and yolk sac it is thought to play an important role in the
endocytosis of many nutrients and lipoproteins (26).
Cubilin binds to a variety of ligands such as albumin (4),
intrinsic factor (IF)-Cbl complex and receptor-associated protein
(5), apolipoprotein A-1 (apoA-1; Refs. 18,
20), transferrin (21), and myeloma light
chains (2). The in vivo role of cubilin in the endocytosis
of the three ligands IF-Cbl, albumin, and apoA-1 is best exemplified in
a canine model that developed vitamin B12 deficiency
(14) due to lack of cubilin expression in the renal and
intestinal apical brush-border membrane (BBM) (15). In
addition to developing vitamin B12 deficiency, these
animals also excreted large amounts of albumin (4) and
apoA-1 (20) in their urine, demonstrating that loss of
renal apical cubilin resulted in a failure of tubular reabsorption of
both apoA-1 and albumin.
Albumin reabsorption by the renal proximal tubular epithelial cells is
an important physiological process, which prevents its urinary
excretion by allowing its uptake by the proximal tubular epithelial
cells. In healthy subjects, albumin filtration and reabsorption are in
equilibrium, and disequilibrium of this process results in albuminuria
(16). Patients with heavy albuminuria are likely to
develop tubulointerstitial inflammation, scarring, and fibrosis and
progress to end-stage renal failure, and such a progression may be
related to slow injury of the epithelial cells (6).
Despite the importance of albumin reabsorption, the role of the large
endocytic receptors cubilin and megalin in this process is not fully
understood. Although cubilin binds to albumin, its endocytosis has been
proposed to depend on interaction of cubilin with megalin, another
large endocytotic receptor of molecular mass 660 kDa (9).
The uptake and endocytosis of albumin by the renal proximal tubular
epithelial cells appear to involve both cubilin and megalin
(41). However, it is not known whether the expression of
both these megareceptors at the apical surface or the interaction
between them regulates the amount of albumin that is reabsorbed by the
proximal tubular epithelial cells. To address some of these issues, we
have used a rat model in which albuminuria was induced after a single
dose of total body irradiation (TBI). Albuminuria noted in these
animals has been suggested to be due to increased glomerulus
permeability of albumin (36), but the effect of radiation
at the tubular reabsorption stage has not been investigated. In our
present study, we have demonstrated that albuminuria noted in these
animals is due to selective loss of albumin and megalin binding, but
not IF-Cbl binding, by renal apical BBM cubilin. In addition,
our study also demonstrates that in these animals, the binding of
megalin to albumin or CIMPR or the binding of cubilin to CIMPR is not
altered significantly, suggesting that under our experimental
conditions and the dose of radiation, the damage to apical membrane
cubilin is highly selective.
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MATERIALS AND METHODS |
Materials.
The following were commercially purchased as indicated:
[57Co]Cbl (1.3 µCi/µg) and carrier free
Na125I (ICN Radiochemicals, Irvine, CA), rat albumin,
protein A, and CNBr Sepharose (Sigma, St. Louis, MO). IF used in these
studies was prepared from the rat stomach as described earlier
(33). Antiserum to purified rat megalin was raised in New
Zealand white rabbits as described earlier (39). Antiserum
to rat renal cubilin was prepared as described earlier
(34). Antiserum to bovine liver CIMPR was prepared as
described earlier (12).
Animals.
The rats used in the study were 9-wk-old WAG/Rij/MCW males that were
bred and housed in Animal Research Center facility at the Medical
College of Wisconsin, Milwaukee, WI. These animals were free of
Mycoplasma pulmonis, Pseudomonas, and common
murine viruses. The protocol used in the study had been reviewed and approved by the Animal Care Committee and the Biohazard Committee of
the Medical College of Wisconsin.
Irradiation.
Animals were given TBI with orthovoltage X-rays. The total radiation
given in a single dose was 9.5 Gy. Unanesthetized animals were
immobilized in a specially constructed Plexiglas jig for irradiation.
Animals received a bone marrow transplant immediately after the end of
the radiation course (27). Control rats were sham
irradiated. Individual irradiated and control rats were kept in
metabolic cages designed to collect urine samples. Urine samples were
collected for a period of 24 h, and the urine collected was divided into small aliquots and frozen at 
70°C. The urine samples were thawed out and used immediately. Some rats were killed at 9 wk
after irradiation, and tissues (kidney and intestine) were removed,
chilled in ice-cold saline for 5 min, and homogenized in 10 mM
Tris · HCl buffer.
Membrane preparations.
Total mucosal membrane from the distal half of the rat intestine was
prepared as follows. Mucosa (1-2 g) suspended in 10-20 ml 10 mM Tris · HCl, pH 7.4, containing 50 mM mannitol, 140 mM NaCl,
0.1 mM phenylmethlsulfonyl fluoride, and 2 mM benzamidine (buffer
A) was homogenized in motor-driven Potter-Elvejhem homogenizer using 10-15 up and down strokes. The homogenate was centrifuged at
100,000 g for 30 min, and the pellet fraction was
resuspended and homogenized in buffer A and used as total
membranes. Apical BBM from rat kidney was prepared by the
Ca2+ precipitation method as described earlier
(35). The yield of the apical BBM marker 
-glutamyl
transpeptidase was ~17% with 15-fold enrichment. Contamination of
the apical BBM by other organelles was between 1 and 2% as determined
by specific marker enzyme assays: 
-glucoronidase (13)
for lysosomes, Na+-K+-ATPase (3)
for basolateral membranes, and NADH oxidase (17) for
microsomal and outer mitochondrial membranes.
Iodination of rat albumin and protein A.
Fifty micrograms of rat serum albumin or protein A was iodinated with
0.5 mCi of Na125I and IODO-GEN as recommended by the
manufacturer. The iodinated rat albumin was separated on a Sephadex
column in 10 mM Tris · HCl buffer, pH 7.4, containing 140 mM
NaCl. The recovery was estimated to be ~80%, and the specific
activity of both albumin and protein A was 2.5-3 × 106
disintegrations · min
1 · µg
protein1.
Ligand binding activity.
Cubilin activity in the kidney BBM was measured by its ability to bind
IF-[57Co]Cbl complex as described earlier
(32). Briefly, rat IF-[57Co]Cbl
(0.3-1.5 pmol) was incubated with 50 µg of rat kidney BBM protein in the presence of 10 mM Tris · HCl buffer, pH 7.4, containing either 5 mM CaCl2 or 5 mM EDTA. The
Ca2+ specific binding of the ligand was calculated as
before (32). 125I-albumin (0.75-40 pmol)
binding was carried out by rapid filtration method (1).
Briefly, ~100 µg of rat kidney BBM protein in 10 mM
Tris · HCl, pH 7.4, containing 140 mM of NaCl was preincubated at 37°C for ~10 min in the presence and absence of 25-fold molar excess of nonradioactive rat serum albumin. Binding of
125I-labeled rat albumin was determined after incubation at
37°C for 1 h. The binding was terminated by the addition of
ice-cold 10 mM Tris · HCl, pH 7.4, containing 140 mM NaCl. The
contents of the binding mixture were rapidly filtered through 0.45-µm
cellulose filters. The tubes were rinsed with 3 ml of the same cold
stop reaction and filtered and counted for filter-bound radioactivity. Specific binding was calculated by subtracting nonspecific
125I-labeled rat albumin binding noted in the presence of
cold rat serum albumin from total 125I-labeled rat
albumin bound to BBM in the absence of nonradioactive rat serum
albumin. The association constant Ka was
determined by the double reciprocal plot according to Hooper et al.
(19).
Preparation of ligand affinity matrix and ligand affinity
chromatography.
Rat serum albumin was coupled to CNBr-activated Sepharose, and rat
gastric IF was coupled to Cbl-Sepharose. One milliliter of a 1:1
suspension in 10 mM Tris · HCl buffer, pH 7.4, of the Sepharose-linked ligands (albumin or IF-Cbl) was capable of binding to
at least 500-700 ng of purified renal cubilin. One hundred micrograms of rat kidney BBM protein was solubilized in 1 ml of buffer
(10 mM Tris · HCl, pH 7.4, containing 140 mM NaCl) containing Triton X-100 (1%). The Triton X-100-solubilized fractions were incubated with 500 µl of 1:1 suspension of Sepharose beads in 10 mM
Tris · HCl, pH 7.4, containing 10 mM CaCl2. After
binding for 60 min, the beads were exhaustively washed with 10 mM
Tris · HCl, pH 7.4, containing 140 mM NaCl (15-20 ml).
Proteins bound were then released by boiling the Sepharose beads with
SDS sample buffer. The released proteins were then subjected to
nonreducing SDS-PAGE.
SDS-PAGE and immunoblotting.
Undiluted rat urine samples from control (50 µl) and irradiated (10 µl) rats or the isolated rat renal BBM (50 µg protein) were
subjected to nonreducing SDS-PAGE (5-7%). In some experiments, the SDS-PAGE of urine samples was stained for protein by Simple Blue
Safe stain from Invitrogen (Carlsbad, CA). Immunoblotting of the
various fractions was carried out as follows. Urine samples or the
eluted fractions from the albumin or IF-Cbl ligand affinity chromatography were subjected to nonreducing SDS-PAGE (5-7%), and
the separated proteins were transferred overnight at 4°C onto Immobilon-P-membrane at constant voltage of 30 V. The membranes were then probed with diluted (1:5,000) antiserum to rat cubilin or
megalin or albumin or to bovine CIMPR and 125I-protein A. The immunoblots were quantified using AMBIS-radioimaging system, and
the intensity of the immunoreacting bands was translated into arbitrary
units. The linearity of the band intensity was confirmed with
immunoblots generated using pure rat renal cubilin or megalin
(200-2,000 ng). The immunoblots are representative data from three
separate blotting experiments using membranes isolated from four or
five animals in each group.
Association of endocytic receptors in the renal BBM.
Association in the BBM of endocytic receptors was carried out
essentially by immunoprecipitation with one antiserum,
followed by SDS-PAGE analysis of immunopellet and finally
immunoblot with antiserum to a different receptor. Isolated
apical renal BBM (100 µg protein) from control and TBI rats was
solubilized in 1 ml of buffer (10 mM Tris · HCl, pH 7.4, containing 140 mM NaCl) containing Triton X-100 (1%). The Triton
X-100-solubilized fraction was subjected to immunoprecipitation with
undiluted (5 µl) cubilin or megalin antiserum and 50 µl of a 1:1
suspension of protein A coupled to Sepharose. The immunopellet was
boiled with SDS sample buffer to release the proteins bound, and the
proteins were then separated on nonreducing SDS-PAGE (5%). The
separated proteins were then transferred overnight at 4°C onto
Immobilon-P-membrane at constant voltage of 30 V. The
membranes were then probed with diluted (1:5,000) antiserum to rat
megalin or bovine CIMPR and 125I-protein A. In the case of
intestine, because of very low levels of cubilin and megalin
expression, total membrane cubilin-megalin association was determined
by immunoprecipitation of Triton X-100 extracts of membrane bound to
IF-[57Co]Cbl with antiserum to cubilin and megalin as
described earlier (39).
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RESULTS |
Albumin in the urine of irradiated rats.
To confirm the presence of albuminuria in the TBI rats, SDS-PAGE
analysis of urine from control and TBI rats was performed (Fig.
1A). The protein pattern on
SDS-PAGE revealed a strong single protein band of molecular mass 66 kDa
in urine of two separate TBI rats (lanes 3 and
4). Low levels of this protein band could also be detected
in the urine of two normal rats (lanes 1 and 2).
Immunoblot analysis (Fig. 1B) with rat albumin antiserum
confirmed that the 66-kDa band was indeed albumin (lane 2),
and this band once again was also detected at low levels in the urine
from control rats (lane 1). These results demonstrated the
presence of strong albuminuria in the TBI rats.
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Fig. 1.
SDS-PAGE and immunoblot analysis of rat urine after total
body irradiation (TBI). Urine from 2 control (lanes 1 and
2) and TBI (lanes 3 and 4) rats was
subjected to nonreducing SDS-PAGE and stained for protein
(A). In some experiments, separated proteins were
transferred onto Immobilon-P-membrane and probed with polyclonal
antiserum to rat serum albumin (B). See MATERIALS AND
METHODS for details.
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Because both cubilin and megalin are large-sized albumin binding
endocytic receptors, they could be the targets for radiation-induced damage that could result in albuminuria due to decreased albumin binding and endocytosis. To test this hypothesis, we first determined the ability of apical BBM to bind albumin, which will be a measure of
its binding to both cubilin and megalin. In addition, we also determined the binding of IF-Cbl to the BBM as this ligand is bound
only by cubilin, but not megalin.
Kinetics of 125I-rat serum albumin and
IF-[57Co]Cbl binding to renal apical BBM from control and
TBI rats.
Ligand binding studies (Table 1) revealed
that albumin binding to the apical BBM isolated from TBI rats declined
by 80% from 50 to 10 pmol/mg protein. The association constant
Ka for BBM binding of albumin increased to 2.5 µM in TBI rats from ~0.5 µM in control rats (Fig.
2). Unlike changes in albumin binding,
IF-Cbl binding to the apical BBM was the same (3.0-3.3 pmol/mg
protein) in both control and TBI rats, and there was no change in the
affinity for IF-Cbl (data not shown). These initial kinetic studies
indicated that either megalin that binds to albumin or cubilin that
binds to both albumin and IF-Cbl may be affected in the renal BBM of TBI rats. To explore these possibilities, the total amount of cubilin
and megalin present in the BBM and the amount of these proteins that
actually bind to albumin and IF-Cbl were determined.
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Fig. 2.
125I-rat serum albumin binding to
brush-border membrane (BBM) of control and TBI rats. Rat kidney BBM
(100 µg) was incubated with varying concentrations (0.75-40
pmol) of 125I-rat serum albumin and incubated at 37°C.
See MATERIALS AND METHODS for details.
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Immunoblot analysis of renal BBM cubilin and megalin.
Immunoblot of renal BBM proteins separated on SDS-PAGE with
monospecific antiserum to rat renal cubilin and megalin (Fig. 3) revealed no significant changes in the
BBM megalin and cubilin protein levels in the TBI (lanes 2 and 4) and control (lanes 1 and 3)
rats. Immunoblot with megalin antiserum did reveal some lower-sized proteins, and these could be degraded products of megalin.
These data coupled with ligand binding data (Table 1) indicated
strongly that TBI might selectively inactivate albumin binding to these
two proteins. To examine this possibility, Triton X-100 extracts of the
BBM were used to purify cubilin by both albumin and IF-Cbl affinity
chromatography and megalin by albumin affinity chromatography.
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Fig. 3.
Immunoblot analysis of BBM megalin and cubilin. BBM from
control (lanes 1 and 3) and TBI (lanes
2 and 4) rats (25 µg protein) was subjected to
nonreducing SDS-PAGE (7%), transferred to Immobilon-P-membrane, and
probed with diluted (1:5,000) polyclonal antiserum to rat cubilin or
megalin and 125I-protein A. The bands were visualized by
autoradiography. Data shown are a typical representative of 4 separate
blots using 8 normal and TBI rat renal BBM.
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Immunoblot analysis of cubilin purified from affinity chromatography
(Fig. 4) using rat serum albumin (Fig.
4A) as a ligand revealed nearly 75% less cubilin present in
the Triton X-100 extracts of BBM from TBI rats (lane 2)
compared with cubilin purified from normal rats (lane 1).
Since albumin binding is also a property of megalin, the same detergent
extracts were used to purify megalin using albumin affinity
chromatography. Immunoblot analysis (Fig. 4A) revealed that
megalin levels purified were the same in both control (lane
3) and TBI (lane 4) rats. Similar immunoblot analysis of
cubilin purified using IF-Cbl as the affinity ligand revealed (Fig.
4B) identical levels of cubilin in Triton X-100 extracts of
BBM from control (lane 2) and TBI rats (lane 1).
In addition to the 460-kDa cubilin band, another band of higher
molecular mass was also detected in the immunoblot using the cubilin
purified from the BBM of both control and TBI rats using IF-Cbl
affinity chromatography. This higher molecular mass protein band was
absent in the purified cubilin fraction purified from the BBM of both control and TBI rats using albumin affinity chromatography.
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Fig. 4.
Immunoblot analysis of cubilin and megalin purified by
affinity chromatography. Triton X-100-solubilized BBM proteins from
control (A, lanes 1 and 3;
B, lane 2) and TBI rats (A,
lanes 2 and 4; B, lane 1)
were bound to Sepharose-rat serum albumin (RSA) or Sepharose-intrinsic
factor-cobalamin (IF-Cbl) column. The proteins bound were released,
subjected to nonreducing SDS-PAGE, transferred to Immobilon-P-membrane,
and probed with diluted (1:5,000) polyclonal antiserum to rat cubilin
or megalin and 125I-protein A. The bands were visualized by
autoradiography. The gel shown is a typical representative of at least
4 experiments carried out using BBM fraction from 4 separate control
and TBI rats.
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Quantitative analysis of the image density of immunoblots (Fig. 4,
A and B) revealed a decline of cubilin protein
levels in the BBM extracts of TBI rats by five- to sixfold relative to
their levels in control rat BBM extracts when these fractions were
subjected to rat serum albumin-Sepharose affinity chromatography (Fig.
5). However, similar quantitation of the
cubilin protein bands purified on IF-Cbl-Sepharose column did not
reveal any significant changes in cubilin protein levels. These results
indicated that in rat renal BBM of TBI rats, the albumin binding region
of cubilin is selectively altered. Although decreased albumin binding
alone can explain the onset of albuminuria in TBI rats, inhibition of endocytosis of residual albumin bound to cubilin may also be inhibited because of TBI, which can damage the formation of the cubilin-megalin complex.
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Fig. 5.
Immunoblots of Fig. 4 were quantified using
AMBIS-radioimaging system, and the intensity of the immunoreacting
bands was translated into arbitrary units. Data represent means ± SD from immunoblots obtained from 4 different experiments.
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Disruption of cubilin-megalin but not CIMPR-megalin association in
the renal BBM of TBI rats.
To determine whether the amount of cubilin associated with megalin is
altered due to irradiation, Triton X-100 extracts of the apical BBM
were subjected to immunoprecipitation with antiserum to cubilin, and
the immune complex was then subjected to immunoblot with antiserum to
megalin. The data (Fig. 6A)
clearly show that cubilin-megalin interaction is disrupted in TBI rat
renal BBM (lane 2), and the loss of this interaction was
~75% compared with control rat BBM (lane 1). Because both
cubilin and megalin are also expressed, but at low levels, in the
distal regions of the rat intestine, we wanted to test whether in TBI
rats intestinal BBM cubilin-megalin association is also disrupted.
Interestingly, we could not detect any significant changes in the
association between cubilin and megalin in the intestinal BBM as nearly
10% of the cubilin-bound IF-[57Co]Cbl could be
immunoprecipitated in the Triton X-100 extracts of BBM from both
control and TBI rats (data not shown). This observation suggested that
under our experimental conditions, TBI damage involving cubilin and
megalin appears to be restricted to renal BBM.
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Fig. 6.
Cation-independent mannose
6-phosphate/insulin-like growth factor II receptor
(CIMPR)-megalin-cubilin interaction. Triton X-100 extract from control
(lanes 1 and 3) and TBI (lanes 2 and
4) rat kidney BBM was first immunoprecipitated with
polyclonal antiserum to rat cubilin (lanes 1 and
2 in A and B) or megalin
(B, lanes 3 and 4) and incubated with
protein A-Sepharose. Bound proteins were separated on nonreducing
SDS-PAGE, transferred to Immobilon-P-membrane, and probed with
polyclonal antiserum to rat megalin or bovine CIMPR and
125I-protein A. The protein bands were visualized by
autoradiography. See MATERIALS AND METHODS for details. IP,
immunoprecipitation; IB, immunoblot.
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To further define the specific nature of the disruption of
cubilin-megalin interaction in the renal BBM of TBI rats, we also tested whether TBI affected the association of megalin with any other
BBM-resident large-sized endocytic receptor. We chose CIMPR, an
endocytic receptor of molecular mass 300 kDa, which has been demonstrated, like megalin, to be localized to the rat renal apical BBM
and in clathrin-coated pits (11). Immunoprecipitation with antisera to either cubilin or megalin followed by immunoblot with CIMPR
antiserum clearly indicated (Fig. 6B) that CIMPR is indeed associated with cubilin (lanes 1 and 2) and
megalin (lanes 3 and 4) and that TBI had no
effect on the association of CIMPR with either cubilin or megalin.
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DISCUSSION |
In the current study, we have investigated the potential role of
cubilin and megalin in the pathogenesis of albuminuria noted in TBI
rats. It is estimated that albumin reabsorption capacity in rats
(30) is about 10-135 mg/l, and in humans nearly
7 g of albumin is reabsorbed within a 24-h period
(7). Defective reabsorption of albumin by the proximal
tubular epithelial cells results in proteinuria and is often preceded
by apical BBM damage. Albuminuria is known to occur in rats during
aging (8), with polycystic kidney disease
(29), in early-stage diabetes (37), and in
rats that are exposed to TBI (36). Although increased glomerulus permeability of albumin has been noted in many causes of
albuminuria, the role of the large albumin receptors megalin and
cubilin expressed in the tubular epithelial apical BBM in the
reabsorption of albumin and pathogenesis of albuminuria is not well understood.
In our rat model, a single dose of TBI resulted in albuminuria as
evidenced by the urinary excretion of albumin (Fig. 1). To understand
the cause of albuminuria in these rats, we focused our studies on the
two albumin binding receptors in the BBM, cubilin and megalin. Cubilin
and megalin, because of their large molecular masses of 460 and 660 kDa, respectively, could be the likely targets for radiation-induced
damage and loss from the BBM. However, immunoblot studies (Fig. 3) did
not reveal any significant changes in their BBM protein levels in
control and TBI rats.
The observation that megalin protein levels (Fig. 3) and its ability to
bind albumin (Fig. 4A, lanes 3 and 4)
were not altered in TBI rats is interesting and suggested strongly that
albumin binding to megalin by itself may not be important for its
tubular reabsorption. Earlier studies in megalin knockout mice have
indicated no significant increase in albuminuria (22), and
only very mild albuminuria was present in the human homolog of murine
megalin deficiency (28). In addition, lack of evidence for
the direct role for megalin in the tubular reabsorption of albumin has
also been shown in rats with early-stage diabetes (37).
Albuminuria in these animals has been proposed to be due to causes such
as increased lipid peroxidation and decreased endocytosis as megalin levels in these rats decreased by only 10% (37). Despite
these studies that have suggested lack of a direct role of megalin in albumin endocytosis, there is evidence from a later study
(4) from megalin knockout mice that albumin excretion in
these animals increased threefold. Taken together, these studies have
suggested that cell surface expression of megalin may play an indirect
role in the endocytosis of albumin, and our data of disruption of
megalin-cubilin interaction in causing albuminuria in TBI rats support
such an indirect role for megalin.
In contrast to megalin, our studies indicate that cubilin plays a more
important role in albumin reabsorption. The following line of evidence
supports such a conclusion. First, albumin binding to BBM was reduced
by nearly 80% (Table 1) without loss of BBM cubilin levels (Fig. 3) in
TBI rat kidney BBM. Second, albumin binding capacity of BBM from TBI
rats is reduced (Fig. 2) by fivefold. Albumin binding kinetic values
(Ka, 0.5 µM; Bmax, 50 pmol/mg
protein) reported in this study using control rat renal BBM are very
close to Kd and Bmax values (0.43 µM and 40 pmol/mg protein, respectively) reported in another study
(1). In addition, the Kd for
albumin binding to rat renal purified cubilin has been reported to be 0.63 µM (4). Finally, the amount of cubilin recovered
from the BBM extracts of TBI rats by albumin affinity chromatography was much lower (75%) than that recovered using extracts obtained from
the BBM of control rats (Fig. 4A, lanes 1 and
2). However, when fractionated on IF-Cbl affinity
chromatography, cubilin levels recovered from both control and TBI rat
BBM extracts were similar (Fig. 4B, lanes 1 and
2). This last observation is interesting as it provides two
important insights into ligand binding properties of cubilin.
Earlier studies (41) based on differential inhibition by
receptor-associated protein of albumin and IF-Cbl binding by cubilin had suggested that IF-Cbl and albumin binding sites could be
distinguished. This suggestion was further supported by our earlier
studies (40), which were based on differential inhibition
of these two ligands binding to cubilin by antiserum to epidermal
growth factor. The present study has confirmed these earlier
suggestions by providing more direct evidence that albumin and IF-Cbl
ligand binding sites of cubilin are different. Two earlier studies have
shown that a small percentage of rat renal BBM cubilin also exists as a
trimer (39) and that purified cubilin in vitro forms
noncovalent trimers connected by NH2-terminal coiled-coil
helix (23). Thus the cubilin band of molecular mass >460
kDa noted when purified from IF-Cbl affinity chromatography (Fig.
4B) could represent functional cubilin trimer that is able
to bind only IF-Cbl, but not albumin, as this band was absent even in
control rat BBM when cubilin was purified by albumin affinity
chromatography (Fig. 4A, lanes 1 and
2). The distinct nature of albumin and IF-Cbl binding sites
of cubilin may help explain why some patients with Grasbeck-Imerslund
syndrome who develop Cbl deficiency due to inherited intestinal
malabsorption of Cbl do not develop proteinuria (10, 26).
It is possible that different mutations of the cubilin molecule may
exist that affect uptake of IF-Cbl, or albumin, or both.
Another interesting aspect of our study is the significant (75%) loss
noted in the amount of cubilin associated with megalin (Fig.
6A, lanes 1 and 2) after a single dose
of TBI. Loss of cubilin-megalin association appears to be specific for
the kidney BBM as it was not detected in the ileal BBM (data not
shown). Furthermore, in the kidney, decreased association of megalin
occurred with cubilin, but not with CIMPR (Fig. 6B). The
specific loss of cubilin-megalin interaction in the renal BBM raises
the question whether the loss of albumin binding by renal cubilin is
due to loss of its association with megalin. However, this is highly
unlikely because cubilin fragments (the 113-residue NH2
terminus or CUB domains 6-8) when expressed in vitro bound albumin
in the absence of megalin (40). Thus, while albumin
binding by cubilin is independent of its interaction with megalin,
their association in the apical BBM appears to play a role in the
endocytosis of albumin and other ligands that bind to cubilin
(25). We have shown earlier (39) that the
NH2-terminal region of cubilin binds to megalin in a
Ca2+-dependent manner. It is not known whether such
interaction with megalin involves any other regions of cubilin. Further
studies are needed to address this issue.
Because of the lack of a transmembrane domain in cubilin
(24), the endocytosis of many of its ligands is thought to
be mediated by its interaction with megalin (25). It is
even suggested that synthesis of megalin (18) is to some
extent (20%) responsible for the cell surface expression of cubilin.
These earlier studies have proposed that megalin acts as a coreceptor
active in the endocytosis and intracellular trafficking of cubilin. The
current data support such a role of megalin by providing evidence for the existence of cubilin-megalin interactions in the native renal BBM
and its importance in the endocytosis of albumin.
In addition to cubilin-megalin interactions in the native BBM, our
results also suggest that CIMPR, another endocytic receptor, also
interacts with both BBM megalin and cubilin (Fig. 6). At present, the
physiological significance, if any, of CIMPR interactions with either
cubilin or megalin in the renal BBM is not known. In this context, it
is interesting to note that in an adult rat male reproductive system,
cubilin endocytosis is mediated via its interaction with low-density
lipoprotein receptor-related protein-2 (38). Thus a
distinct possibility exists that CIMPR could under some conditions
function as a coreceptor for renal cubilin. However, this possibility
is unlikely as far as endocytosis of cubilin-bound albumin is concerned
because reduced albumin reabsorption was noted in megalin knockout mice
(4). Despite our current lack of understanding of the
physiological importance of interactions of CIMPR with cubilin or
megalin, to the best of our knowledge, this study is the first to
demonstrate the association of cubilin and megalin with CIMPR in the
rat renal BBM. On the basis of this finding, we propose a model (Fig.
7) to illustrate the functional
topography of these three endocytic receptors, two of which, megalin
and CIMPR, contain both a transmembrane domain and a COOH-terminal
cytoplasmic tail.
View larger version (46K):
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|
Fig. 7.
A proposed model for megalin-cubilin and CIMPR
interaction in the rat kidney BBM. The BBM orientation of the 3 endocytic receptors cubilin, megalin, and CIMPR (not drawn to a scale
representing their molecular mass) is indicated. Arrowhead indicates
the albumin binding sites on cubilin (2 sites) and megalin (location
and number not determined). The black arrow encompassing the 3 receptors indicates mutual interaction among them.
|
|
In summary, these studies have shown that albumin and megalin binding
by renal apical BBM cubilin play an important role in the endocytosis
of filtered albumin and that megalin plays only an indirect role in
this process. Further studies are needed to address the issues
regarding 1) the effect on cubilin interactions with albumin
and megalin in other causes of albuminuria and 2) the
structural basis for the albumin and megalin binding by cubilin in
health and disease.
| |
ACKNOWLEDGEMENTS |
This work was supported by U.S. Dept. of Veterans Affairs Grant
7816-01P awarded to B. Seetharam.
| |
FOOTNOTES |
Address for reprint requests and other correspondence: B. Seetharam, MACC Fund Center Rm. 6061, Medical College of Wisconsin, 8701 Watertown Plank Rd., Milwaukee, WI 53226 (E-mail:
seethara{at}mcw.edu).
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.
April 4, 2002;10.1152/ajpregu.00752.2001
Received 20 December 2001; accepted in final form 2 April 2002.
| |
REFERENCES |
1.
Bakala, H,
Perichon M,
Sudey I,
and
Schaverbeke J.
Binding of 125I-labeled albumin by isolated rat renal brush-border membrane vesicles. Evidence for uptake and internalization process.
Int J Biochem
22:
1189-1194,
1990[Web of Science][Medline].
2.
Batuman, V,
Verroust PJ,
Navar GL,
Kaysen JH,
Goda FO,
Campbell WC,
Simon E,
Pontillon F,
Lyles M,
Bruno J,
and
Hammond TG.
Myeloma light chains are ligands for cubilin (gp280).
Am J Physiol Renal Physiol
275:
F246-F254,
1998[Abstract/Free Full Text].
3.
Beauge, L,
Berberian G,
and
Campos M.
Potassium-p-nitrophenyl phosphate interactions with (Na+/K+)-ATPase. Their relevance to phosphatase activity.
Biochim Biophys Acta
773:
157-164,
1984[Medline].
4.
Birn, H,
Fyfe JC,
Jacobsen C,
Mounier F,
Verroust PJ,
Orskov H,
Willnow TE,
Moestrup SK,
and
Christensen EI.
Cubilin is an albumin binding protein important for renal tubular albumin reabsorption.
J Clin Invest
105:
1353-1361,
2000[Web of Science][Medline].
5.
Birn, H,
Verroust PJ,
Nexo E,
Hager H,
Jacobsen C,
Christensen EI,
and
Moestrup SK.
Characterization of an epithelial ~460-kDa protein that facilitates endocytosis of intrinsic factor-vitamin B12 and binds receptor-associated protein.
J Biol Chem
272:
26497-26504,
1997[Abstract/Free Full Text].
6.
Brunskill, N.
Mechanisms of albumin uptake by proximal tubular cells.
Am J Kidney Dis
37, Suppl2:
17-20,
2001.
7.
Brunskill, NJ,
Stuart J,
Tobin AB,
Walls J,
and
Nahoorski S.
Receptor-mediated endocytosis of albumin by kidney proximal tubule cells is regulated by phosphatidylinositide 3-kinase.
J Clin Invest
101:
2140-2150,
1998[Web of Science][Medline].
8.
Cessac, AL,
Perichon M,
Schaverbake J,
and
Bakala H.
Age-related changes in albumin binding by renal brush-border membrane vesicles.
Mech Ageing Dev
70:
139-148,
1993[Web of Science][Medline].
9.
Christensen, EI,
and
Birn H.
Megalin and cubilin: synergistic endocytic receptors in the renal proximal tubule.
Am J Physiol Renal Physiol
280:
F562-F573,
2001[Abstract/Free Full Text].
10.
Collan, Y,
Lahdevirta J,
and
Jokinen EJ.
Selective vitamin B12 malabsorption with proteinuria.
Nephron
23:
297-303,
1979[Web of Science][Medline].
11.
Cui, S,
Flyvbjerg A,
Nielsen S,
Kiess W,
and
Christensen EI.
IGF-II/Man-6-P receptors in rat kidney: apical localization in proximal tubule cells.
Kidney Int
43:
796-807,
1993[Web of Science][Medline].
12.
Dahms, NM,
Brzycki-Wessell MA,
Ramanujam KS,
and
Seetharam B.
Characterization of mannose 6-phosphate receptors (MPRs) from opossum liver: opossum cation-independent MPR binds insulin-like growth factor-II.
Endocrinology
133:
440-446,
1993[Abstract/Free Full Text].
13.
Dean, RT.
Rabbit -glucuronidase, subcellular distribution and immunochemical properties.
Biochem J
138:
407-410,
1974[Web of Science][Medline].
14.
Fyfe, JC,
Jezyk PF,
Giger U,
and
Patterson DF.
Inherited selective malabsorption of vitamin B12 in giant schnauzers.
J Am Anim Hosp Assoc
25:
533-539,
1989.
15.
Fyfe, JC,
Ramanujam KS,
Ramaswamy K,
Patterson DF,
and
Seetharam B.
Defective brush-border expression of intrinsic factor-cobalamin receptor in canine inherited intestinal cobalamin malabsorption.
J Biol Chem
266:
4489-4494,
1991[Abstract/Free Full Text].
16.
Gekle, M.
Renal proximal tubular albumin reabsorption: daily prevention of albuminuria.
News Physiol Sci
13:
5-11,
1998[Abstract/Free Full Text].
17.
Gimenez, GG,
Benavides J,
Garcia ML,
and
Valdivieso F.
Occurrence of a reduced nicotinamide adenine dinucleotide oxidase activity linked to a cytochrome system in renal brush border membrane.
Biochemistry
19:
4834-4839,
1980[Medline].
18.
Hammad, SM,
Barth JL,
Knaak C,
and
Argraves WS.
Megalin acts in concert with cubilin to mediate endocytosis of high density lipoproteins.
J Biol Chem
275:
12003-12008,
2000[Abstract/Free Full Text].
19.
Hooper, DC,
Alpers DH,
Burger RL,
Mehlman CS,
and
Allen RH.
Characterization of ileal vitamin B12 binding using homogeneous human and hog intrinsic factor.
J Clin Invest
52:
3074-3083,
1973[Web of Science][Medline].
20.
Kozyraki, R,
Fyfe J,
Kristiansen M,
Gerdes C,
Jacobsen C,
Cui S,
Christensen EI,
Aminoff M,
de la Chapelle A,
Krahe R,
Verroust PJ,
and
Moestrup SK.
The intrinsic factor-vitamin B12 receptor, cubilin, is a high-affinity apolipoprotein A-I receptor facilitating endocytosis of high-density lipoprotein.
Nat Med
5:
656-661,
1999[Web of Science][Medline].
21.
Kozyraki, R,
Fyfe J,
Verroust PJ,
Jacobsen C,
Dautry-Varsat A,
Gburek J,
Willnow TE,
Christensen EI,
and
Moestrup SK.
Megalin-dependent cubilin-mediated endocytosis is a major pathway for the apical uptake of transferrin in polarized epithelia.
Proc Natl Acad Sci USA
98:
12491-12496,
2001[Abstract/Free Full Text].
22.
Leheste, JR,
Rolinski B,
Vorum H,
Hilpert J,
Nykjaer A,
Jacobsen C,
Aucouturier P,
Moskaug JO,
Otto A,
Christensen EI,
and
Willnow TE.
Megalin knockout mice as an animal model of low molecular weight proteinuria.
Am J Pathol
155:
1361-1370,
1999[Abstract/Free Full Text].
23.
Lindblom, A,
Quadt N,
Marsh T,
Aeschlimann D,
Morgelin M,
Mann K,
Maurer P,
and
Paulsson M.
The intrinsic factor-vitamin B12 receptor, cubilin, is assembled into trimers via a coiled-coil alpha-helix.
J Biol Chem
274:
6374-6380,
1999[Abstract/Free Full Text].
24.
Moestrup, SK,
Kozyraki R,
Kristiansen M,
Kaysen JH,
Rasmussen HH,
Brault D,
Pontillon F,
Goda FO,
Christensen EI,
Hammond TG,
and
Verroust PJ.
The intrinsic factor-vitamin B12 receptor and target of teratogenic antibodies is a megalin-binding peripheral membrane protein with homology to developmental proteins.
J Biol Chem
273:
5235-5242,
1998[Abstract/Free Full Text].
25.
Moestrup, SK,
and
Verroust PJ.
Megalin and cubilin-mediated endocytosis of protein-bound vitamins, lipids, and hormones in polarized epithelia.
Annu Rev Nutr
21:
407-428,
2001[Web of Science][Medline].
26.
Mohamed, SD,
McKay E,
and
Galloway WM.
Juvenile familial megaloblastic anemia due to selective malabsorption of vitamin B12.
QJM
139:
433-453,
1966.
27.
Moulder, JE,
and
Fish BL.
Late toxicity of total body irradiation with bone marrow transplantation in a rat model.
Int J Radiat Oncol Biol Phys
16:
1501-1509,
1989[Web of Science][Medline].
28.
Muller, D,
Ankermann T,
Stephani U,
Kirschstein M,
Szelestei T,
Luft FC,
and
Willnow TE.
Holoprosencephaly and low molecular weight proteinuria: the human homologue of murine megalin deficiency.
Am J Kidney Dis
37:
624-628,
2001[Web of Science][Medline].
29.
Obermuller, N,
Kranzlin B,
Blum W,
Gretz N,
and
Witzgall R.
An endocytosis defect as a possible cause of proteinuria in polycystic kidney.
Am J Physiol Renal Physiol
280:
F244-F253,
2001[Abstract/Free Full Text].
30.
Oken, DE,
and
Flamenbaum W.
Micropuncture studies of proximal tubule albumin concentration in normal and nephrotic rats.
J Clin Invest
50:
1498-1505,
1971[Web of Science][Medline].
31.
Seetharam, B.
Receptor-mediated endocytosis of cobalamin (vitamin B12).
Annu Rev Nutr
19:
173-195,
1999[Web of Science][Medline].
32.
Seetharam, B,
Alpers DH,
and
Allen RH.
Isolation and characterization of the ileal receptor for intrinsic factor-cobalamin.
J Biol Chem
256:
3785-3790,
1981[Free Full Text].
33.
Seetharam, B,
Bakke JE,
and
Alpers DH.
Binding of intrinsic factor to ileal brush border membrane in the rat.
Biochem Biophys Res Commun
15:
238-244,
1983.
34.
Seetharam, B,
Levine JS,
Ramasamy M,
and
Alpers DH.
Purification, properties, and immunochemical localization of a receptor for intrinsic factor-cobalamin complex in the rat kidney.
J Biol Chem
263:
4443-4449,
1988[Abstract/Free Full Text].
35.
Seetharam, S,
Ramanujam KS,
and
Seetharam B.
Synthesis and brush border expression of intrinsic factor-cobalamin receptor from rat renal cortex.
J Biol Chem
267:
7421-7427,
1992[Abstract/Free Full Text].
36.
Sharma, M,
Sharma R,
Ge XL,
Fish BL,
McCarthy ET,
Savin VJ,
Cohen EP,
and
Moulder JE.
Early detection of radiation-induced glomerular injury by albumin permeability assay.
Radiat Res
155:
474-480,
2001[Web of Science][Medline].
37.
Tojo, A,
Onozato ML,
Ha H,
Kurihara H,
Sakai T,
Goto A,
Fujita T,
and
Endou H.
Reduced albumin reabsorption in the proximal tubule of early-stage diabetic rats.
Histochem Cell Biol
16:
269-276,
2001.
38.
Van Praet, O,
Argraves WS,
and
Morales CR.
Co-expression and interaction of cubilin and LRP-2 in the adult male rat reproductive system.
Mol Biol Cell
12:
A487,
2001.
39.
Yammani, RR,
Seetharam S,
and
Seetharam B.
Cubilin and megalin expression and their interaction in the rat intestine: effect of thyroidectomy.
Am J Physiol Endocrinol Metab
281:
E900-E907,
2001[Abstract/Free Full Text].
40.
Yammani, RR,
Seetharam S,
and
Seetharam B.
Identification and characterization of two distinct ligand binding regions of cubilin.
J Biol Chem
276:
44777-44784,
2001[Abstract/Free Full Text].
41.
Zhai, XY,
Nielsen R,
Birn H,
Drumm K,
Mildenberger S,
Freudinger R,
Moestrup SK,
Verroust PJ,
Christensen EI,
and
Gekle M.
Cubilin- and megalin-mediated uptake of albumin in cultured proximal tubule cells of opossum kidney.
Kidney Int
58:
1523-1533,
2000[Web of Science][Medline].
Am J Physiol Regul Integr Comp Physiol 283(2):R339-R346
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