(Received for publication, August 31, 1996, and in revised form, October 16, 1996)
From the Department of Cell and Developmental Biology, Oregon Health Sciences University, Portland, Oregon 97201-3098
Cell-surface receptors that undergo clathrin-mediated endocytosis contain short amino acid sequences in their cytoplasmic domain that serve as internalization signals. Interactions between these sequences and components of the endocytic machinery should become limiting upon overexpression of the constitutively recycling transferrin receptor (TfR). A tetracycline-responsive system was used to induce overexpression of the TfR up to 20-fold in HeLa cells. Internalization assays indicate the rate of 125I-transferrin uptake per surface TfR is reduced by a factor of 4 in induced cells. Consistent with endocytosis being the rate-limiting step, TfRs shift from an endosomal to more of a plasma membrane distribution with TfR overexpression. The clathrin-associated protein AP-2 has been proposed to interact directly with the cytoplasmic domain of many receptors, yet no changes in the amount or distribution of AP-2 were detected in induced cells. The internalization rate for the epidermal growth factor receptor was also measured, with or without induction of TfR expression. Even though endocytosis of the TfR is saturated in induced cells, 125I-labeled epidermal growth factor continues to be internalized at a rate identical to that seen in uninduced cells. We propose that there are different limiting steps for the endocytosis of these two receptors.
Receptor-mediated endocytosis is a mechanism by which a number of cell-surface receptors and their ligands are internalized by the cell. The process involves the concentration of specific plasma membrane proteins into clathrin-coated pits, followed by rapid internalization and delivery to early endosomes. The exact mechanism by which sequestration of surface receptors occurs is unclear, although it appears that short amino acid sequences in the cytoplasmic domains of captured proteins act as internalization signals that are necessary and in some cases sufficient for endocytosis (1-8).
Internalization signals have been identified for a large number of
proteins that span several different classes of receptors (reviewed in
Ref. 9). A common tyrosine-based motif, which has been proposed to form
secondary structure comprising a -turn, provides a potential
functional link between these signals. The structurally similar signals
are believed to interact directly with proteins of the coated pit,
presenting the possibility of competition for internalization among
receptors. The clathrin-associated protein AP-2 has been proposed to be
the primary candidate for interacting with the cytoplasmic domains of
receptors targeted for internalization (10-13).
We are investigating the mechanisms by which receptors are recruited to clathrin-coated pits. Using the tetracycline-responsive promoter cell expression system developed by Gossen and Bujard (14), we show that by overexpressing an epitope-tagged TfR1 in HeLa cells, the endocytic mechanism can be saturated such that the rate of internalization for Tf per surface TfR decreases at high TfR concentrations. The expression and distribution of AP-2 remain unaltered in induced cells. Additionally, we demonstrate that although the pathway of endocytosis for TfR is saturated, the activated EGFR continues to be internalized at a rate similar to that in uninduced cells. We conclude that there are different limiting steps for the endocytosis of these two receptors.
The plasmid pCD-TR1, containing the sequence for the human TfR, was a gift from Dr. A. McClelland (Yale University) (15). The pUHD10-3 plasmid was a gift from Drs. M. Gossen and H. Bujard (Zentrum für Molekulare Biologie, Universität Heidelberg) (14).
Subcloning and Site-directed MutagenesisThe human TfR cDNA coding region in pCD-TR1 is contained within a 2.5-kilobase BamHI-XbaI fragment. A HindIII site 900 bases from the start codon was used to generate the 1.5-kilobase HindIII-XbaI fragment, which was subsequently cloned into the M13mp18 vector for mutagenesis. The oligonucleotide-directed mutagenesis system (Amersham Corp.) was used to insert the sequence for the flag epitope (-DYKDDDDK-) (16) immediately prior to the termination codon. The modified C-terminal portion of the human TfR was excised with HindIII-BamHI and ligated with the BamHI-HindIII N-terminal fragment into the pUHD10-3 BamHI site, resulting in the fTfR/pUHD10-3 construct.
IodinationEither 1600 µg of human holo-Tf (Intergen Co.) or 5 µg of human EGF (Life Technologies, Inc.) was used in a 50-µl reaction of 225 mM sodium phosphate buffer (pH 7.0), 0.5 units of lactoperoxidase (Sigma), 2 mCi of carrier-free Na125I (DuPont NEN), and 0.003% H2O2 (Sigma). The mixture was allowed to react for 5 min at room temperature before adding 50 µl of 2% blue dextran in phosphate-buffered saline. The protein was separated from unreacted Na125I on a 2-ml desalting column (Pierce).
ImmunodetectionCells grown on coverslips were washed
several times with phosphate-buffered saline, fixed for 15 min at room
temperature with 3% paraformaldehyde, and washed an additional two
times with phosphate-buffered saline (17, 18). Cells on coverslips were
incubated for 1 h at room temperature with a 1:50 dilution of
sheep anti-TfR antibody (characteristics similar to goat anti-TfR
antibody described earlier (19)), followed by a second 1-h incubation
at room temperature with a 1:50 dilution of fluorescein
isothiocyanate-labeled swine anti-goat secondary antibody (Tago, Inc.).
Reducing SDS-polyacrylamide gel electrophoresis and Western blotting
were as described previously (20). An anti-peptide antibody (1868) to
the eight-amino acid flag epitope sequence coupled to keyhole limpet
hemocyanin was generated in rabbits and affinity-purified
(Immuno-Dynamics, Inc., La Jolla, CA). Molecular mass markers
(Sigma) included myosin heavy chain (205 kDa),
-galactosidase (116 kDa), phosphorylase b (97 kDa),
bovine serum albumin (68 kDa), ovalbumin (43 kDa), and carbonic
anhydrase (29 kDa).
The fTfR20-2 cell line was generated by introducing the fTfR/pUHD10-3 plasmid into tTA HeLa cells (provided by Dr. Sandra L. Schmid, Scripps Research Institute) by calcium phosphate precipitation (21). Selection was achieved by cotransfecting with pBSpac (22), which contains the resistance gene for the antibiotic puromycin. All colonies were recloned to ensure a pure cell line. Selected colonies were screened by gel electrophoresis and Western blot analysis with 1868 rabbit anti-flag and sheep anti-TfR primary antibodies.
Transfected cells (fTfR20-2 cells) were maintained in Dulbecco's modified Eagle's medium supplemented with 10% fetal bovine serum, 400 µg/ml G418 (Geneticin), 400 ng/ml puromycin, and 2 µg/ml tetracycline. To induce overexpression of the TfR, tetracycline was excluded from the medium, and cells were allowed to grow for at least 96 h (unless otherwise indicated).
Uptake ProtocolThe rate of 125I-Tf uptake was
measured using a method modified from McGraw and Maxfield (23).
fTfR20-2 cells grown to confluency in six-well plates
(1-2 × 106/well) were washed twice with wash medium
(Dulbecco's modified Eagle's medium buffered with 20 mM
HEPES (pH 7.4)) and incubated for 15 min at 37 °C. At time 0, 1 ml
of either medium S (wash medium + 210 nM
125I-Tf) or medium NS (medium S + 1 mg/ml unlabeled Tf) was
added to four wells or two wells of a six-well plate, respectively. Each plate was incubated at 37 °C and 5% CO2 for 2, 4, 6, or 8 min, after which it was placed on ice and incubated with an
acidic buffer (0.2 N acetic acid, 0.2 M NaCl)
for 2 min at 4 °C to remove any surface-bound 125I-Tf.
Each well was washed four times with 4 °C final wash medium (150 mM NaCl, 20 mM HEPES (pH 7.4), 1 mM
CaCl2, 5 mM KCl, and 1 mM
MgCl2); solubilized in 0.1 N NaOH, 0.1% Triton
X-100; and counted on a -counter. The counts represent only the
125I-Tf that was internalized during the 37 °C
incubation. The number of surface TfRs for each uptake experiment was
determined by incubating four wells and two wells of a six-well plate
in medium S and medium NS, respectively, on ice for 90 min. These wells
were washed four times with 4 °C final wash medium and solubilized
as described above. All results were corrected for specific
measurements by subtracting nonspecific uptake and binding amounts. TfR
distribution was determined following the protocol described by McGraw
and Maxfield (23), except that 125I-Tf was used at a higher
concentration (210 nM).
fTfR20-2 cells were grown to
confluency on six-well plates pretreated with poly-D-lysine
(Sigma). To expose the cytoplasmic face of the
membrane, cells were freeze-fractured by placing plates on ice for 15 min, washing once with 1 ml of H2O at 4 °C, and placing
at 80 °C with 1 ml of H2O for ~1 h. While thawing in a 37 °C bath, each well was brought to a final concentration of Buffer E (36.4 mM HEPES, 68.2 mM KCl, 4.1 mM magnesium acetate (pH 7.2), 1 mM
dithiothreitol, 10 µM leupeptin (Sigma),
1 mM ortho-phenanthroline (Sigma), 0.5 mM benzamidine
(Sigma), and 2 µg/ml soybean trypsin inhibitor
(Sigma)) (24) or Buffer F (0.5 M Tris-Cl
(pH 7.0), 10 µM leupeptin, 1 mM
ortho-phenanthroline, 0.5 mM benzamidine, 2 µg/ml soybean trypsin inhibitor, and 1 mM dithiothreitol)
(25). Attached membranes were scraped from the wells, and the pooled samples were centrifuged at 1600 × g for 10 min at
4 °C, followed by centrifugation of the supernatant at 90,000 × g for 45 min at 4 °C. Membrane pellets and whole cell
lysates were solubilized in NET buffer (150 mM NaCl, 5 mM EDTA (pH 7.4), and 10 mM Tris-Cl) + 1%
Triton X-100. Samples representing equal numbers of cells were run on
an SDS-polyacrylamide (8%) gel and transferred to nitrocellulose.
Western blots were probed with either a mouse monoclonal antibody to
AP-2 (clone 100/2; Sigma) or sheep anti-TfR antibody,
followed by horseradish peroxidase-conjugated swine anti-mouse and
swine anti-goat antibodies (Boehringer Mannheim), respectively.
A cell line capable of overexpressing the TfR was needed to study the effect of TfR density on endocytosis. The tetracycline-responsive promoter system developed by Gossen and Bujard (14) was chosen because the expression of the TfR could be tightly controlled. The system involves the use of a stable HeLa cell line that expresses a fusion protein consisting of the tetracycline-responsive element (tetR) from Escherichia coli and the VP16 activation domain from herpes simplex virus. In the absence of tetracycline, the tTA is free to bind tetracycline operator sequences found in the promoter region of the pUHD10-3 plasmid and to promote transcription. When tetracycline is added to the cell medium, the tTA fusion protein is blocked from interacting with the promoter, and transcription does not occur.
The human TfR sequence containing a flag epitope tag at its carboxyl
terminus (C-flag TfR) was subcloned into the pUHD10-3 vector. The
fTfR/pUHD10-3 construct along with a puromycin selection vector (pBSpac
(22)) were cotransfected into tTA-expressing HeLa cells. Approximately
30 colonies were isolated and screened by Western analysis for
inducible expression of the C-flag TfR in the absence of tetracycline
in the medium. Induction of the C-flag TfR (94 kDa) along with a minor
amount of unreduced TfR (180 kDa) was detected in two different clones
using the anti-flag antibody (Fig. 1, right
panel). Since the promoter region by itself is silent in mammalian
cells, no detectable expression of the C-flag TfR is seen at day 0. Anti-TfR antibody shows endogenous levels of wild-type TfR at day 0 of
induction and a distinct increase in total TfRs (wild-type and C-flag
TfRs) after 3-4 days (Fig. 1, left panel). Clone
fTfR20-2 was used in subsequent experiments.
Before quantitative 125I-Tf uptake measurements of the
fTfR20-2 clone as a population could be made, we wanted to
show that expression of the C-flag TfR was homogeneously induced in all
of the cells. fTfR20-2 cells were grown in either the
absence or presence of tetracycline to represent induced or uninduced
cells, respectively. Surface TfR expression was visualized by
incubating nonpermeabilized fixed cells with a fluorescein
isothiocyanate-conjugated polyclonal antibody to the TfR. A more
intense surface fluorescence labeling is apparent in induced cells
(Fig. 2, Tet), indicating a greater number
of TfRs. This level of fluorescence was seen uniformly in all cells for
every microscopic field observed. Uninduced cells (Fig. 2,
+Tet) display a labeling pattern identical to that of the
parent tTA HeLa cell line (data not shown), indicating full repression
of the C-flag TfR protein.
Stable fTfR20-2 Cells Can Be Induced to Express C-flag TfR at Levels 10-20-fold over Endogenous TfR
The binding of Tf
was examined to quantitate the actual number of TfRs being expressed on
the cell surface of the fTfR20-2 clone. Scatchard analysis
was performed on uninduced and induced fTfR20-2 cells (Fig.
3). Uninduced cells show binding sites equivalent to
~1.5-2.0 × 105 TfRs/cell surface and a
Kd of Tf for the TfR of 3.1 nM.
Cell-surface binding sites on the order of 2.0-4.0 × 106 TfRs/cell, a factor of 10-20-fold increase over
endogenous TfR, are measured in induced cells. The
Kd of Tf for the TfR measured in induced cells is
lower (25.8 nM), suggesting that addition of the flag
epitope to the C terminus affects Tf binding to a limited extent. All
uptake assays were done at 210 nM 125I-Tf to
ensure that the uptake assays reflected the rate of uptake, and not the
rate of Tf binding. Bindings performed with either 210 or 420 nM 125I-Tf yielded similar results, indicating
that Tf binding was saturating and not the limiting factor in the
uptake experiments (data not shown).
Rate of Tf Uptake per Surface TfR Is Decreased in Induced fTfR20-2 Cells
Rates of 125I-Tf uptake
were measured to demonstrate that the induction of TfR expression in
the fTfR20-2 cell line is sufficient to saturate
endocytosis. Uninduced or induced cells were incubated with a
saturating amount of 125I-Tf (210 nM) for 2, 4, 6, or 8 min at 37 °C and 5% CO2. Uninduced fTfR20-2 cells expressing 2 × 105
TfRs/cell surface display an endocytic rate of 0.39 Tf
molecules/surface TfR/min (Fig. 4). In induced cells
(2 × 106 TfRs/cell surface), the measured rate was
0.10 Tf molecules/surface TfR/min, a significant 3.9-fold decrease.
Control uptakes were performed on the parent tTA HeLa cell line, grown
with or without tetracycline, to demonstrate that the effects we have
measured were specific to the number of TfRs expressed on the surface. No significant difference in the rate of 125I-Tf
endocytosis was detected (data not shown).
The number of TfRs expressed on the surface was compared with the rate
of 125I-Tf uptake per surface TfR to determine whether
endocytosis of the TfR could be saturated. We needed to vary the length
of time that fTfR20-2 cells spend in the absence of
tetracycline to control the number of TfRs, but it was difficult to
completely remove all of the tetracycline from plated cells by washing,
resulting in sporadic induction. In contrast, turning off expression by plating induced cells onto six-well plates and adding tetracycline for
varying periods of time gave more precise control over TfR number.
Immediately following tetracycline addition, the number of TfRs on the
cell surface decreased at a rate reflective of the half-life of the
receptor. Uptake of 125I-Tf was measured 12-72 h after
repressing TfR synthesis. Fig. 5 shows the compiled
results from two experiments. Each point represents one uptake assay
from which an endocytic rate and surface TfR number were determined.
Although the rate of endocytosis of 125I-Tf increases with
levels of TfR expression up to 20-fold over endogenous levels, the
relationship is not linear, but rather appears to saturate at surface
TfR densities >1 million. These results imply that the endocytosis of
the TfR becomes limiting at these higher receptor concentrations.
Proportion of TfRs on the Cell Surface Increases with TfR Overexpression
If the TfR is internalized at a slower rate per
surface TfR in induced cells and TfR recycling remains the same, then a
change in the distribution of receptors from the internal compartments to the cell surface should be apparent. The TfR distribution changes after a 10-fold induction of surface receptor number (from 2 × 105 to 2 × 106 TfRs/cell surface) from a
surface/internal ratio of 1:4 for uninduced fTfR20-2 cells
to a ratio of 1:1 for induced fTfR20-2 cells (Fig. 6). The surface/internal ratio for uninduced
fTfR20-2 cells is identical to the distribution seen in the
parent tTA HeLa cell line (data not shown). These results are
consistent with the idea that TfRs recycling back to the plasma
membrane at a normal rate will have to wait for a longer period of time
to be internalized by a saturated endocytic system.
Rate of EGF Uptake per EGFR Is Unchanged between Uninduced and Induced Cells
We wanted to determine how overexpression of the
constitutively recycling TfR would affect the endocytosis of a
triggered receptor, such as the EGFR. The EGFR has been shown to
colocalize with the TfR in coated pits after binding its ligand, EGF
(26, 27), making it a potential competitor with the TfR for common endocytic components. Using the same protocol as described for TfR
uptake, we examined the rate of internalization of 125I-EGF
in induced and uninduced fTfR20-2 cells (Fig.
7). Although induced cells express nearly 2 million TfRs
on the cell surface, a density that we have shown to impede the
endocytosis of the TfR, the rate of endocytosis of the EGFR is not
significantly changed from that of uninduced cells (compare 0.17 with
0.16 EGF molecules/surface EGFR/min). This result suggests that they do not share a common rate-limiting factor(s) or pathway.
Distribution of the Clathrin Adaptor Protein AP-2 Remains Unchanged in Cells Overexpressing TfR
Tyrosine-based motifs in the cytoplasmic domains of a number of receptors are involved in the concentration of these receptors into coated vesicles (1, 5, 6, 28, 29). AP-2, a major component of the clathrin-coated pit, has been shown to interact specifically with a number of receptors and peptides targeted for internalization (12, 30-36). Using electron microscopy to quantitate their results, both Iacopetta et al. (28) and Miller et al. (37) have noted that either more clathrin-coated pits or more clathrin lattices are associated with the plasma membrane of cells expressing high numbers of TfR than in corresponding cells with fewer TfRs. If more clathrate structures are associated with the plasma membrane, then more AP-2 should be associated, too.
We were interested to see whether a large number of TfRs on the cell
surface would lead to a redistribution of AP-2 to the plasma membrane,
as might be expected if AP-2 interacts with the cytoplasmic domain of
the TfR. The amount of AP-2 either attached to the membrane or present
in the cytosol was measured in both uninduced and induced cells to
determine the AP-2 distribution (Fig. 8). Using a
protocol modified from Mahaffey et al. (25), cells were
freeze-fractured to expose the cytoplasmic face and thawed in either a
control buffer (Buffer E), which preserves AP-2 and clathrin binding to
membranes, or a Tris buffer (Buffer F) to dissociate clathrin and
adaptor proteins from the membrane and to show the total amount of AP-2
in the cells. Cells were fractionated into pellet
(P)-containing membranes and supernatant (S)-containing cytosol by scraping and centrifugation.
Samples representing an equal number of cells were subjected to
SDS-polyacrylamide gel electrophoresis, transferred to nitrocellulose,
and immunodetected with an antibody to AP-2 or TfR. The levels of AP-2
seen in the membrane (pellet) fractions of uninduced or induced
fTfR20-2 cells washed with Buffer E are similar. No AP-2
was detected in membranes washed with Buffer F, indicating that AP-2
could be removed from the membranes as described previously (25). A
direct comparison of whole cell lysates demonstrated that the overall
levels of AP-2 expression remain unchanged, regardless of the number of TfRs. We conclude that AP-2 is not actively recruited to the plasma membrane with increased TfR expression and that other factors control
or limit the association of AP-2 with the plasma membrane.
The mechanism by which specific plasma membrane proteins are selected for endocytosis by clathrin-coated pits has recently been a subject of great interest. Since many internalization signals on the cytoplasmic domains of proteins that are endocytosed through this mechanism share similar structural motifs, it is attractive to suggest that a common recognition protein is involved. The adaptor protein complex AP-2 has been proposed to be the "recruiter" protein (11). AP-2 is directly involved in the recruitment of clathrin to the membrane and potentiates the formation of clathrin structures. Early evidence that AP-2 interacts with cytoplasmic domains of receptors targeted for internalization came from work that described its specific association with an affinity matrix column composed of the internalization signal-containing cytoplasmic domains of either the low density lipoprotein receptor or the mannose 6-phosphate receptor (11, 33). The ability of the cytoplasmic domains of internalizing receptors (low density lipoprotein receptor, mannose 6-phosphate receptor, and immunoglobulin receptor) to elute AP-2 from the affinity column lent support to the idea that AP-2 was a common component of the endocytic mechanism. Co-immunoprecipitation studies revealed a strong interaction between AP-2 and activated EGFR (38, 39). In contrast, recent evidence suggested that the high affinity binding of AP-2 to the EGFR was not necessary for efficient internalization of the EGFR (30, 32). No measurable binding of AP-2 to the cytoplasmic domain of the TfR has been demonstrated, although interactions between the tetrapeptide internalization sequence of the TfR and the µ-subunit of AP-2 have been detected using the two-hybrid system and surface plasmon resonance (13).
Generation of a cell line capable of overexpressing a single cycling receptor, specifically the TfR, should slow the endocytosis of other receptors if indeed there is a common protein involved with the coated pit recognition mechanism. The present set of experiments demonstrates that overexpression of the TfR does saturate some rate-limiting step or component of its own endocytosis. In uninduced fTfR20-2 cells as well as in the parent tTA HeLa cell line, an average of 1.50 × 105 TfRs are on the cell surface, and Tf is internalized at a rate of 0.39 Tf molecules/surface TfR/min. When fTfR20-2 cells are induced, the surface TfR population increases to between 2 and 4 × 106 surface TfRs/cell, and a decreased rate of as low as 0.10 Tf molecules internalized per surface TfR/min is measured.
Our finding that the endocytosis of a constitutively cycling receptor can be saturated is at odds with the proposal that only the endocytosis of triggered receptors is saturable. The idea that the endocytosis of constitutively recycling receptors is not saturable at high receptor concentrations arose from two observations. First, two reports about coated pit formation in cells with high numbers of TfRs have been published. Iacopetta et al. (28) used electron microscopy to demonstrate that high TfR densities led to an increase in the number of coated pits forming at the plasma membrane. Miller et al. (37) presented evidence that although an increase in flat clathrin lattice area was apparent in cells with high numbers of TfRs, the actual number of coated pits remained constant. These results imply that receptors recruit AP-2 and clathrin to the plasma membrane. We did not detect any redistribution of AP-2 from the cytosol to the plasma membrane or any increase in AP-2 or clathrin concentrations (data not shown) in cells under conditions in which we see comparable numbers of TfRs (the induction of TfR is 10-20-fold and the rate of 125I-Tf uptake per surface TfR is decreased 4-fold). Second, Rothenberger et al. (40) reported that no changes in the rate of 125I-Tf endocytosis per surface TfR were detected in mouse cells expressing large numbers of human TfRs (4.6 × 106) versus lower numbers of TfRs (~1.5 × 105), although the uptake rate of 59Fe per TfR decreased. They concluded that exocytosis rather than endocytosis slowed at high TfR numbers. No changes in the rate of exocytosis of the TfR were detected in our system. Our results imply that TfRs do not actively recruit adaptor proteins to the plasma membrane, but rather the TfRs diffuse to or aggregate in pre-existing coated pits and that this process can be saturated.
The reasons why our results differ from the previous results are not totally obvious. The method that we used to observe the association of AP-2 with the plasma membrane has been shown by several groups to reflect an accurate AP-2 distribution (12, 25, 41). The method of measuring 125I-Tf uptake differs from that of Rothenberger et al. (40) in that our assay does not include prebinding Tf at 4 °C before allowing uptake to occur at 37 °C. Perhaps, the initial rates of endocytosis that Rothenberger et al. measured could have been affected by the cells recovering from a low temperature block of endocytosis.
The idea that the cytoplasmic domains of receptors do not directly recruit AP-2 to the plasma membrane is consistent with recent work by Santini and Keen (42). Using an immobilized antigen for IgE Fc receptors, they were able to show receptor activation without internalization, which led to an aggregation of receptors at the exposed surface. No discernible difference in the level or distribution of either clathrin or AP-2 between activated and inactive receptors was detected. Together with our data, this suggests that AP-2 recruitment and coated pit formation are regulated independently of receptor concentrations.
The lack of competition that we have seen between the EGFR and the TfR for endocytosis is consistent with earlier experiments. Using A431 cells that normally express a high density of many types of receptors, Wiley demonstrated that internalization of the EGFR could be saturated (43). Since the EGFR is a triggered receptor, it does not cluster into coated pits until it binds EGF. By modifying the amount of EGF given to cells, the effective concentration of active EGFR in the coated pits could be increased, and the rate of internalization measured. Although saturation of the endocytosis of the EGFR was obvious, the rate of TfR internalization was unaffected. Studies of Lamaze et al. (44) demonstrated that endocytosis of the EGFR and the TfR has different biochemical requirements.
In summary, we show that overexpression of a single recycling receptor can overwhelm endocytosis such that the rate of internalization per receptor decreases. This saturation, which is dependent on the surface receptor number, reflects a limiting factor for TfR internalization. In addition, we show that the rate of internalization for the EGFR does not change with the induction of TfR expression. This supports the idea that there are at least two different rate-limiting steps in the endocytosis of these two receptors. Finally, we show that the overall distribution and expression level of AP-2 remain the same, independent of receptor number.
The system described in this paper provides a valuable resource for
examining specific interactions of the cytoplasmic domains of
internalizing receptors with members of the endocytic machinery. In the
case of the TfR, we are studying a single tyrosine-based sorting motif.
This type of signal has been shown to be important for the
internalization of a number of other membrane proteins, such as TGN38
(45), the asialoglycoprotein receptor (46), the low density lipoprotein
receptor (5, 36), and vesicular stomatitis virus protein G (47). Many
membrane proteins have multiple possible endocytic signals, such as the
insulin receptor -subunit, which has two tyrosine-based signals in
tandem (48). The cation-dependent mannose 6-phosphate
receptor has a tyrosine-based as well as a dileucine-based sorting
motif (49, 50), as do the EGFR (51) and the glucose 4 transporter (52).
Often, the signals that are being utilized are difficult to dissect
using site-directed mutagenesis. Internalization-deficient mutants
could result from an indirect effect of destroying tertiary or
quaternary structure of the entire cytoplasmic domain, rather than from
the desired effect of altering the endocytic signal. Our system allows us to saturate the system with one receptor and to quantitatively look
for competition in vivo with unaltered endogenous
receptors.