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© The Rockefeller University Press, 0021-9525/2003/10/155 $8.00
The Journal of Cell Biology, Volume 163, Number 1, 155-164

MAL regulates clathrin-mediated endocytosis at the apical surface of Madin–Darby canine kidney cells

¹ Centro de Biología Molecular "Severo Ochoa", Universidad Autónoma de Madrid and Consejo Superior de Investigaciones Científicas, Cantoblanco, Madrid, 28049 Spain
² Departamento de Biología Celular, Facultad de Medicina, Universidad de Murcia, Murcia, 30071 Spain

Address correspondence to Miguel A. Alonso, Centro de Biología Molecular "Severo Ochoa", Universidad Autónoma de Madrid and Consejo Superior de Investigaciones Científicas, Cantoblanco, Madrid, 28049 Spain. Tel.: 34-91-397-8037. Fax: 34-91-397-8087. email: maalonso{at}cbm.uam.es

	Abstract

Top Abstract Introduction Results Discussion Materials and methods References

 

MAL is an integral protein component of the machinery for apical transport in epithelial Madin–Darby canine kidney (MDCK) cells. To maintain its distribution, MAL cycles continuously between the plasma membrane and the Golgi complex. The clathrin-mediated route for apical internalization is known to differ from that at the basolateral surface. Herein, we report that MAL depends on the clathrin pathway for apical internalization. Apically internalized polymeric Ig receptor (pIgR), which uses clathrin for endocytosis, colocalized with internalized MAL in the same apical vesicles. Time-lapse confocal microscopic analysis revealed cotransport of pIgR and MAL in the same endocytic structures. Immunoelectron microscopic analysis evidenced colabeling of MAL with apically labeled pIgR in pits and clathrin-coated vesicles. Apical internalization of pIgR was abrogated in cells with reduced levels of MAL, whereas this did not occur either with its basolateral entry or the apical internalization of glycosylphosphatidylinositol-anchored proteins, which does not involve clathrin. Therefore, MAL is critical for efficient clathrin-mediated endocytosis at the apical surface in MDCK cells.

Key Words: apical endocytosis; protein machinery; polarized transport; epithelial cells; lipid rafts

Abbreviations used in this paper: FR, folate receptor; GPI, glycosylphosphatidylinositol; NHS-SS-biotin, sulfosuccinimidyl 2-(6-(biotinamido)hexanoamido)ethyl-1-3'-dithiopropionate; pIgR, polymeric Ig receptor; sulfo-NHS-biotin, sulfo-N-hydroxyl-succinimido-biotin.

	Introduction

Top Abstract Introduction Results Discussion Materials and methods References

 
In polarized epithelial cells, the composition of the apical and basolateral membrane subdomains is maintained by specialized exocytic and endocytic pathways that sort newly synthesized and internalized proteins, respectively, specifically to each surface subdomain (Mostov et al., 2000). Clathrin-mediated endocytosis takes place at both the apical and basolateral domains but the process differs at both membrane surfaces (Naim et al., 1995). The mechanisms of exocytic transport are also different for each membrane surface (Matter and Mellman, 1994). In epithelial MDCK cells, sorting to the basolateral surface is mediated by sequences in the cytoplasmic tail of membrane proteins that might or might not be related to tyrosine- and dileucine-based sorting signals (Mellman et al., 1993). In contrast, a direct pathway of transport to the apical membrane appears to be mediated by integration of cargo proteins into specialized glycolipid-enriched membrane microdomains or rafts (Simons and Wandinger-Ness, 1990).

MAL is a raft-associated integral membrane protein of 17 kD, which has been demonstrated to be an essential element of the machinery for efficient apical transport in MDCK cells (Cheong et al., 1999; Puertollano et al., 1999; Martin-Belmonte et al., 2000, 2001). Despite the intense vesicular traffic to deliver newly synthesized apical cargo, MAL accumulation at the plasma membrane is prevented by continuous recycling to the Golgi complex via the endosomal system, which, in addition, allows its participation in new rounds of cargo transport (Puertollano and Alonso, 1999). At steady state, 12% of MAL is detected in the plasma membrane including clathrin-coated pits and buds in MDCK cells (Puertollano et al., 2001). Here, we have analyzed the clathrin requirement for MAL internalization and investigated the role of MAL in the internalization of apical proteins. As model proteins, we used the polymeric Ig receptor (pIgR) and the transferrin receptor, which are known to internalize from both the apical and basolateral surface through a clathrin-mediated pathway (Odorizzi et al., 1996; Altschuler et al., 1999), and glycosylphosphatidylinositol (GPI)-anchored proteins, such as placental alkaline phosphatase and folate receptor (FR), which use clathrin-independent mechanisms (Nichols and Lippincott-Schwartz, 2001). Our results indicate that MAL uses clathrin for apical endocytosis and that MAL is required for internalization of pIgR and transferrin receptor from the apical, but not from the basolateral, surface or apical endocytosis of GPI-anchored proteins.

	Results

Top Abstract Introduction Results Discussion Materials and methods References

 
Apical endocytosis of MAL takes place by a clathrin-dependent pathway in MDCK cells
To detect MAL on the cell surface and to track its internalization, we prepared stable transfectants of MDCK cells (MDCK/MAL-FLAG cells) that stably expressed a MAL protein bearing a FLAG tag in its last extracellular/luminal loop (MAL-FLAG). The tag makes MAL-FLAG accessible to anti-FLAG antibodies from the extracellular space (Puertollano and Alonso, 1999). To interfere with clathrin-mediated endocytosis, we transiently expressed GFP-DPF coil, an EH-deleted form of the Eps 15 protein tagged with the GFP, which behaves as a dominant-negative mutant and provokes a block of clathrin-coated pit endocytosis (Benmerah et al., 1999). MDCK/MAL-FLAG cells were transfected with GFP-DPF coil, plated, and left to polarize for 48 h in tissue culture filter inserts. The transepithelial resistance of the cell monolayer was measured to ensure proper tight junction formation. As a control for cell polarization, the distributions of gp135 and E-cadherin, chosen as apical and basolateral markers, respectively, were determined in parallel cultures. Fig. 1 A shows that, consistent with the presence of MAL in surface clathrin pits and buds (Puertollano et al., 2001), overexpression of GFP-DPF coil led to a complete block of MAL-FLAG apical internalization. As controls, we observed in parallel that overexpression of GFP-DPF coil halted the apical internalization of pIgR (Fig. 1 B) but did not affect that of FR (Fig. 1 C) in MDCK/pIgR and MDCK/FR cells that stably express pIgR and FR, respectively. Quantitative analysis showed that the great majority of cells positive for GFP-DPF coil were defective for endocytosis of MAL and pIgR (Fig. 1 D), whereas they remained competent at internalizing the GPI-anchored FR molecule. Antibody internalization was demonstrated by examining x-z sections of the cells (Fig. 1 A, MAL-FLAG) and by resistance to acid washes (unpublished data). Finally, as a further control, we observed that endocytosis of all MAL-FLAG, pIgR, and FR (unpublished data) was blocked by expression of a dynamin mutant, dyn^K44A, defective in GTP binding and hydrolysis (Damke et al., 1994), which impairs both clathrin-dependent and -independent pathways (McNiven et al., 2000).

View larger version (48K): [in this window] [in a new window]   Figure 1. Effect of a dominant-negative mutant of Eps15 on apical internalization of MAL. MDCK/MAL-FLAG, MDCK/pIgR or MDCK/FR cells, which stably express MAL-FLAG, pIgR and FR, respectively, were transiently transfected with GFP-DPF coil cDNA. The cells were plated onto tissue culture filters and left to polarize for 48 h at 37°C. Cells were incubated with (A) Alexa-594–labeled anti-FLAG, (B) anti-pIgR, or (C) anti-FR antibodies from the apical surface at 4°C for 30 min, washed, and fixed (time 0) or shifted to 37°C for 30 min to allow internalization before fixation. Cells were then analyzed by confocal immunofluorescence microscopy. Optical x-y and x-z sections are presented in A, whereas only x-y sections are shown in B and C. As an internal control, internalization of MAL-FLAG and pIgR was observed in cells not expressing GFP-DPF coil (arrowheads). MAL-FLAG internalization in the absence of GFP-DPF coil is clearly detected in the corresponding x-z view (arrowhead). FR internalized regardless of the expression of GFP-DPF coil. Note that, although the cell monolayer was tightly confluent, only the cells expressing the exogenous products are stained. As a control of polarization, the cell monolayers were stained after fixation and permeabilization for gp135 and E-cadherin, as markers for the apical and basolateral surface, respectively. Bar, 10 µm. (D) The percentage of untransfected (black bars) and GFP-DPF coil-transfected (gray bars) cells with internalized MAL-FLAG, pIgR or FR is shown. The values shown are the mean of three independent replicates. Greater than 100 cells from each case were analyzed.

View larger version (84K): [in this window] [in a new window]   Figure 2. Time-lapse confocal microscopic analysis of MAL and pIgR internalization. MDCK/pIgR cells were transiently transfected with GFP-MAL and grown on coverslips. 48 h after transfection, cells were incubated at 4°C for 30 min with antibodies anti-pIgR coupled to Alexa-594, and then shifted to 37°C. Sequential images of GFP-MAL and pIgR bound to the antibody were acquired at 5-s intervals using a confocal fluorescence microscope (see Video 1, available at http://www.jcb.org/cgi/content/full/jcb.200304053/DC1). The left panel shows two membrane regions (1 and 2) selected to illustrate endocytic vesicles in which pIgR and GFP-MAL cointernalization was detected (right panels). Some representative frames obtained in a plane close to the coverslip are shown. The time frame intervals are indicated. The outlined circles and the arrowheads label single vesicles carrying both GFP-MAL and pIgR. Bar, 10 µm.

View larger version (43K): [in this window] [in a new window]   Figure 3. Double-label confocal analysis of endocytic vesicles in polarized MDCK cells. MDCK cells stably expressing MAL-FLAG and pIgR were plated onto culture filters and incubated at 37°C for 72 h. Anti-FLAG and anti-pIgR antibodies were coupled to Alexa-488 and Alexa-594, respectively, and applied to the cell monolayers from the apical (A) or the basal (B) side at 4°C for 30 min. Cells were then washed, and shifted at 37°C for 3 min to allow internalization. Cells were fixed and analyzed by confocal microscopy. Images of a (A) subapical x-y plane, an (B) x-y plane corresponding to the contact of the basal surface with the filter, and x-z sections obtained from different fields are shown. Note in the x-z sections that, when the antibodies are added to the apical or basal side, only vesicles in the proximity of the respective cell surface are labeled with no detectable staining in the lateral domains as the antibodies cannot access to them in vivo. Arrows indicate examples of vesicles positively labeled for MAL and pIgR after apical internalization. Bar, 10 µm. (C) Quantitative analysis of pIgR-containing vesicles derived from the apical or the basal surface screened for the simultaneous presence of internalized MAL-FLAG is shown.

View larger version (120K): [in this window] [in a new window]   Figure 4. Colocalization studies of MAL with endocytosed pIgR by immunoelectron microscopy. (A) MDCK cells expressing MAL-FLAG and pIgR were allowed to internalize the pIgR bound to antibodies and to 10-nm-diam protein A–gold (see Material and methods) for 3 min at 37°C. Analysis of ultrathin cryosection revealed that the receptor–antibody–protein A–gold complex was located at restricted areas of the plasma membrane, pits, and endocytic vesicles. Arrowheads point to a clathrin-coated vesicle containing the internalized receptor complex. (B–E) Ultrathin sections of cells treated as described in A but double immunolabeled for MAL, which is visualized by using antitag antibodies and 15-nm-diam protein A–gold. The micrographs show examples of MAL and pIgR colocalization at the (B) plasma membrane, (C) clathrin-coated pits, (D) clathrin-coated vesicles, and (E) uncoated vesicles. Note the characteristic clathrin coats (arrowheads) in C and D. All micrographs shown were taken at the same magnification. Bar, 200 nm.

View larger version (72K): [in this window] [in a new window]   Figure 5. Effect of MAL depletion on apical endocytosis. MDCK cells stably expressing (A and C) pIgR, (B) FR, (D) gD1-DAF, or (E) normal cells were transfected with either antisense oligonucleotide AS or control oligonucleotide AM, plated on tissue culture inserts and incubated at 37°C for 48 h. (A) Cells were incubated at either the apical or the basal side with anti-pIgR antibodies for 30 min at 4°C and then at either 4°C or 37°C for 30 min (apical endocytosis) or at either 4°C for 60 min or at 37°C for 10 min followed by incubation at 18°C for 50 min (basolateral endocytosis) to accumulate the pIgR internalized from the basal side in apical endosome compartments (Apodaca et al., 1994). The cells were fixed, permeabilized or not with Triton X-100 (TX100), and incubated with fluorescent secondary antibodies. (B) Cells were incubated at the apical side with anti-FR antibodies coupled to Alexa-594 for 30 min at 4°C. Cells were fixed or incubated at 37°C for 120 min and then fixed and processed for confocal fluorescence microscopy. (C) Cells were incubated at the apical side with anti-pIgR antibodies and protein A coupled to 10-nm-diam gold particles for 30 min at 4°C. After extensive washings, cells were incubated for 30 min at 37°C, fixed and processed for conventional immunoelectron microscopy. Only the result obtained with the cells treated with the oligonucleotide AS is shown. The complex accumulated in clathrin-coated pits with normal morphology (arrowheads). Bar, 200 nm. (D) Cells were incubated at the apical side with anti-gp135 antibodies for 30 min at 4°C and the bound antibody was detected with a fluorescent secondary antibody (left). The apical content of gD1-DAF and gp114 at steady state was determined by labeling with sulfo-NHS-biotin. The new arrival of gD1-DAF at the apical membrane was determined as described in Materials and methods. The intensity of the signals was quantified and is represented in arbitrary units (right). (E) Cells were incubated at the apical side with dog transferrin for 30 min at 4°C. After washing, cells were incubated for 30 min at either 4°C or 37°C to prevent or allow endocytosis, respectively. The cells were then fixed, permeabilized or not with Triton X-100, and sequentially incubated with antitransferrin antibodies and fluorescent secondary antibodies. Bar, 10 mm. In A, B, D, and E, the images shown are of an apical or a basal frame (4°C), to visualize antibody binding, or from a composite projection of all the frames (37°C and 37°C–18°C), to monitor internalization. Endocytosed material is highlighted by arrowheads in A, B, and E.

To analyze the effect of MAL depletion further, the apical internalization of the pIgR molecule was also investigated by biochemical means (Fig. 6). MDCK/pIgR cells were transfected with either antisense oligonucleotide AS or control oligonucleotide AM and plated in tissue culture inserts. After 48 h at 37°C, the apical surface was labeled at 4°C with sulfosuccinimidyl 2-(6-(biotinamido)hexanoamido)ethyl-1-39-dithiopropionate (NHS-SS-biotin), a reducible analogue of sulfo-N-hydroxyl-succinimido-biotin (sulfo-NHS-biotin). Cells were then incubated for 30 min at 37°C to allow internalization and the biotin label that remained on the cell surface was removed by treating the cells with glutathione, leaving the endocytosed label protected from the reducing agent (Lisanti et al., 1990). After immunoprecipitation, internalized pIgR was visualized by immunoblotting with streptavidin peroxidase. An example of the efficiency of the glutathione treatment is shown in the left panel of Fig. 6 A. The vast majority (>90%) of apical pIgR was endocytosed after 30 min in control MDCK cells (Fig. 6 A, top left), whereas only a minor portion (<5%) was internalized (Fig. 6 A, top middle) in cells with whose MAL levels were reduced to 5% of those in control cells, as quantified by densitometric scanning of the immunoblots obtained with anti-MAL mAb 2E5 (Fig. 6 B). To confirm that these effects were due to MAL depletion and not to spurious effects of the antisense oligonucleotide, we used MDCK/MAL-N cells expressing a truncated form of human MAL (MAL-N) that is resistant to the depletion treatment as its mRNA cannot pair with the antisense oligonucleotide (Fig. 6 B, right; Martin-Belmonte et al., 2000). The exogenous expression of MAL-N allowed normal apical endocytosis of pIgR (Fig. 6 A, right) despite the drop in the amount of endogenous MAL (Fig. 6 B, left). A quantitative analysis of the effect of MAL depletion on apical internalization of pIgR is shown in Fig. 6 C.

View larger version (33K): [in this window] [in a new window]   Figure 6. Biochemical analysis of the effect of MAL depletion on apical endocytosis of the pIgR. (A) MDCK or MDCK/MAL-N cells stably expressing pIgR were transfected with either antisense oligonucleotide AS or control oligonucleotide AM and plated on tissue culture inserts. After 48 h at 37°C, the apical surface was labeled with NHS-SS-biotin, and the cells were incubated at 4°C or 37°C. After 30 min, the label remaining on the cell surface was removed by glutathione treatment. After immunoprecipitation with specific antibodies, internalized pIgR was visualized by immunoblotting with streptavidin peroxidase. (B) Endogenous MAL levels were quantified by densitometric scanning of the immunoblots of the initial lysates with anti–dog MAL 2E5 mAb (left). As the anti–dog MAL antibody does not react with the human protein (Puertollano et al., 1999), tagged human MAL was detected with antitag antibodies (right). One representative experiment out of six performed is shown. (C) Quantitative analysis of the effect of MAL depletion on apical endocytosis of pIgR. The intensity of the protein bands obtained in the different experiments was quantified by densitometric analysis. The values shown are the mean values expressed as a percentage of the biotinylated pIgR present on the apical surface at 4°C in the absence of glutathione treatment.

	Discussion

Top Abstract Introduction Results Discussion Materials and methods References

A direct role or a secondary effect?
The reduction of MAL content slows down the delivery of apical cargo but apical transport is not completely ablated, probably because of the remaining MAL molecules (Puertollano et al., 1999; Martin-Belmonte et al., 2000). As a consequence of this "leaky" transport, the steady-state content of apical proteins is similar in both normal and MAL-depleted MDCK cells (Martin-Belmonte et al., 2000). Consistent with this, we observed similar levels of FR, placental alkaline phosphatase, gD1-DAF, gp135, and gp114 in the apical membrane regardless of the levels of MAL, although we have previously shown that GPI-anchored cargo proteins and transmembrane proteins require MAL for efficient apical transport (Martin-Belmonte et al., 2000). Therefore, although it cannot be ruled out, it is unlikely that MAL depletion reduces specifically the steady-state apical levels of a hypothetical cargo molecule important for apical endocytosis of pIgR but not for that of GPI-anchored proteins. The simplest explanation for all our observations is that the reduction of the MAL content directly affects apical internalization of pIgR.

MAL as machinery for the formation of clathrin-coated apical endocytic vesicles
The observations that (1) MAL is required for apical transport (Cheong et al., 1999; Puertollano et al., 1999; Martin-Belmonte et al., 2000); (2) apical cargo accumulates in the Golgi complex in MDCK cells with reduced levels of MAL (Cheong et al., 1999; Martin-Belmonte et al., 2001); and (3) overexpression of MAL results in de novo formation of a large number of intracellular vesicles (Puertollano et al., 1997), led to the proposal that MAL is an element of the machinery involved in the formation of apical transport vesicles. We have not observed significant differences in the initial processes of pIgR clustering and formation of coated pits at the apical surface between normal MDCK cells and cells with reduced levels of MAL, although an accumulation of the pIgR in clathrin pits and buds was observed at later times in MAL-depleted cells, which is consistent with apical internalization of the pIgR being blocked by MAL depletion. We have recently demonstrated that MAL2, a novel raft protein of the MAL family (Perez et al., 1997), is essential for the exit of vesicular carriers from perinuclear endosomes so that they may travel to the apical membrane during transcytotic transport in hepatoma HepG2 cells (de Marco et al., 2002). It has been proposed that synaptophysin, a tetraspan protein of the physin family, participates in the biogenesis of the synaptic vesicles (Thiele et al., 2000; Huttner and Zimmerberg, 2001). It is of note that MAL family proteins share a protein sequence motif, referred to as the MARVEL motif, with physins and gyrins that it is thought to play a role in membrane trafficking (Sánchez-Pulido et al., 2002). Therefore, we find it plausible that MAL, the other members of the MAL family, and probably other proteins containing a MARVEL domain could serve as machinery for lipid remodelling during biogenesis of transport vesicles. Consistent with this, our present results indicate that MAL is essential for the process of clathrin-mediated internalization of the pIgR in the raft-enriched apical surface and that the maturation process of apical-coated pits to produce vesicles appears to be impaired in cells with reduced levels of MAL.

	Materials and methods

Top Abstract Introduction Results Discussion Materials and methods References

 
Materials
The mouse hybridoma that produces mAb 9E10 to the c-Myc epitope was purchased from the American Type Culture Collection. Rabbit polyclonal antibodies to pIgR were purchased from DakoCytomation (Glostrup). Peroxidase-conjugated anti–mouse or anti–rabbit IgG antibodies, peroxidase-coupled streptavidin, NHS-SS-biotin, sulfo-N-hydroxyl-succinimido-phenyl-propionate, and sulfo-NHS-biotin were purchased from Pierce Chemical Co. Fluorochrome-conjugated secondary antibodies were purchased from Southern Biotechnology Associates, Inc. The Alexa fluor–488 and –594 antibody labeling kits were from Molecular Probes. The anti–human FR antibodies and the human FR cDNA construct were donations from L. Kremer (Centro Nacional de Biotecnología, Madrid, Spain); the antibodies to the gp135 and gp114 apical markers were gifts from E. Rodriguez-Boulan (Cornell University, New York, NY). The anti–dog transferrin antibodies were donated by K. Mostov (University of San Francisco, San Francisco, CA). Anti-FLAG M2 antibodies and dog transferrin were obtained from Sigma-Aldrich. Protein A–gold was obtained from the Department of Cell Biology at Utrecht University.

Cell culture conditions, transfections, and DNA constructs
Epithelial MDCK II cells were grown on Petri dishes, glass coverslips, or tissue culture inserts in DME supplemented with 10% FBS (Sigma-Aldrich), 50 units/ml penicillin, and 50 µg/ml streptomycin, at 37°C in an atmosphere of 5% CO₂/95% air.

The MAL-FLAG construct, encoding MAL modified at its last extracellular loop by insertion of the sequence DYKDDDDK, which contains the FLAG epitope (DYKD), and the construct expressing a human MAL protein lacking the four amino acids contiguous with the initial methionine residue and bearing the 9E10 c-Myc epitope (MAL-N) have been described previously (Puertollano and Alonso, 1999; Martin-Belmonte et al., 2000). The construct expressing MAL fused at its amino terminus to GFP (GFP-MAL) was generated by cloning a DNA fragment with the MAL coding sequence, except the ATG translation initiation site, in-frame with the last codon of the GFP coding sequence contained in the pEGFP-C1 DNA vector (BD Biosciences). Transfections were done by electroporation using an electroporation instrument (model ECM 600; BTX). Selection of stable MDCK cell transfectants was performed by treatment with either 0.5 mg/ml G418 sulfate (Sigma-Aldrich), or 0.5 µg/ml puromycin (Sigma-Aldrich) for 4 wk after transfection. Drug-resistant clones were picked up with cloning rings, and individual clones were screened by immunofluorescence analysis with the appropriate antibodies. The clones that proved to be positive were maintained in drug-free medium. After several passages through this medium, 60–70% of cells within the selected positive clones retained expression of the exogenous product. The 19-mer phosphorothioate oligonucleotide AS, complementary to canine MAL mRNA, and the oligonucleotide control AM, similar in composition to AS but with some replacements to prevent pairing with endogenous MAL mRNA, have been described previously (Puertollano et al., 1999; Martin-Belmonte et al., 2000). The GFP-DPF coil DNA construct, the EH deleted form of the Eps15 protein coupled to GFP was a gift of A. Sorkin (University of Colorado, Denver, CO).

Domain-selective labeling with biotin-containing reagents
For separate access to apical or basolateral domains, MDCK cells were seeded at confluent levels on 24-mm polyester tissue culture inserts of 0.4 µm pore size (Transwell; Costar Inc.). The integrity of the cell monolayer was monitored by measuring the transepithelial electrical resistance using the Millicell ERS apparatus (Millipore). To follow the endocytosis of pIgR and FR, we used the protocol described previously by Lisanti et al. (1990). In brief, 0.5 mg/ml NHS-SS-biotin was added either to the apical or basolateral compartment of the filter chamber. After 30 min at 4°C, the solution was removed and remaining unreacted biotin quenched by incubation with ice cold serum-free culture medium. Cells were then incubated at 37°C in prewarmed normal medium to allow endocytosis. At the indicated times, the biotin label remaining on the cell surface was stripped by reduction with two sequential treatments with 50 mM glutathione at 4°C. Cell monolayers were extensively washed and extracted with 0.5 ml of 25 mM Tris-HCl, pH 7.5, 150 mM NaCl, 5 mM EDTA, 1% Triton X-100, and 60 mM octyl-glucoside for 30 min on ice. Extracts were immunoprecipitated, and fractionated by SDS-PAGE. Biotinylated proteins were detected by immunoblotting with streptavidin peroxidase.

The steady-state levels of gD1-DAF and gp114 at the apical surface of MDCK cells stably expressing exogenous gD1-DAF were determined by labeling the apical surface with 0.5 mg/ml sulfo-NHS-biotin. To determine the delivery of gD1-DAF to the apical surface, cells were pretreated at the apical compartment with 0.5 mg/ml sulfo-N-hydroxyl-succinimido-phenyl-propionate, which lacks the biotin moiety, for 10 min to quench free amino groups. The solution was removed and the treatment was repeated five times to quench residual free amino groups (Lisanti et al., 1990). After incubation for 7 h at 37°C, the appearance of newly delivered molecules on the cell surface was monitored by domain-selective labeling with sulfo-NHS-biotin. Finally, lysates were subjected to immunoprecipitation with the appropriate antibody coupled to protein G–Sepharose, and immunoblotting with streptavidin peroxidase. Using this procedure, it was determined previously that 95% of the newly arrived population of gD1-DAF is due to biosynthetic delivery, whereas the remaining 5% may represent a recycling pool (Lisanti et al., 1990).

Immunoprecipitation and immunoblot analyses
For use in immunoprecipitation studies, antibodies were prebound overnight to protein G–Sepharose in 10 mM Tris-HCl, pH 8.0, 0.15 M NaCl, and 1% Triton X-100 at 4°C. Postnuclear supernatants, prepared with 1% Triton X-100 plus 60 mM octyl-glucoside, were incubated at 4°C for 4 h with a control antibody bound to protein G–Sepharose. After centrifugation, the supernatant was immunoprecipitated by incubation 4°C for 4 h with the appropriate antibody bound to protein G–Sepharose. The immunoprecipitates were collected, washed six times with 1 ml of 10 mM Tris-HCl, pH 8.0, 0.15 M NaCl, and 1% Triton X-100, and fractionated by SDS-PAGE. For immunoblot analysis, samples were transferred to Immobilon-P membranes (Millipore) and blocked with 5% nonfat dry milk and 0.05% Tween 20 in PBS. The blots were then incubated with the indicated primary antibody. After several washings, blots were incubated for 1 h with secondary anti-IgG antibodies coupled to HRP, washed extensively, and developed using an ECL Western blotting kit (Amersham Biosciences).

Immunofluorescence and time-lapse confocal microscopic analyses
For immunofluorescence microscopy, cells grown on culture filters or on coverslips were washed twice with PBS, fixed in 4% PFA for 15 min, rinsed, and treated with 10 mM glycine for 10 min to quench the aldehyde groups. Then, cells were permeabilized or not with 0.2% Triton X-100 and were incubated with 3% BSA for 20 min. After incubation with the appropriate primary and secondary antibodies, images were obtained using a confocal laser microscope (model radiance 2000; Bio-Rad Laboratories) or a conventional fluorescence microscope (Carl Zeiss MicroImagining, Inc.). In some of the experiments presented here, a specific fluorescent primary antibody was used in living cells to monitor internalization and the cells were processed for immunofluorescence analysis directly after fixation. For time-lapse confocal fluorescence microscopy, MDCK cells expressing GFP-MAL and pIgR grown on coverslips were incubated with anti-pIgR antibodies coupled to Alexa-594 for 30 min at 4°C, washed, and incubated at 37°C in a thermal-controlled chamber coupled to the confocal microscope. GFP-MAL and pIgR images were transferred to a computer workstation running MetaMorph imaging software (Universal Imaging Corp.). Cells images were captured at 5-s intervals using a 63x lens. Controls to assess the specificity and the lack of cross-labeling, included incubations with control primary antibodies or omission of either of the primary antibodies.

Immunoelectron microscopy
MDCK/MAL-FLAG/pIgR cells grown on culture filters were incubated at the apical side with anti-pIgR antibodies followed by protein A coupled to 10-nm gold particles, extensively washed and incubated at 37°C for 3 min. Thereafter, the cells were fixed 2 h with 2% PFA and 0.2% glutaraldehyde in 0.1 M phosphate buffer, removed from the filters, and processed for cryosectioning as described previously (Martínez-Menárguez et al., 1999, 2001). In brief, the cells were collected by centrifugation, embedded in 10% gelatin, and cut into small blocks. The blocks were infused overnight with 2.3 M sucrose, mounted in aluminum pins, frozen in liquid nitrogen, and stored until cryoultramicrotomy. Ultrathin cryosections were immunolabeled with antitag antibody followed by a bridging rabbit anti–mouse IgG antibody and protein A coupled to 15-nm gold particles. For conventional electron microscopic studies, normal or MAL-depleted cells grown on culture filters were incubated at the apical side with anti-pIgR antibodies followed by protein A coupled to 10-nm gold particles, extensively washed and incubated for either 2 or 30 min at 37°C. Cells were then fixed for 2 h with 2% PFA and 0.2% glutaraldehyde, fixed after for 2 h with 1% osmium, and embedded in Epon using standard techniques. To quantify the relative distribution of the internalized pIgR–antibody–protein A–gold complex, ultrathin sections of Epon-embedded normal and MAL-depleted MDCK cell monolayers were scanned directly along their apical portion under the electron microscope at a magnification of 20,000. Gold particles (n > 200) were ascribed to one of the after categories: plasma membrane (excluding coated pits), clathrin-coated pits and vesicles, and the rest of endocytic membranes (noncoated vesicles and endosomes). The number of gold particles found over each compartment was expressed as percentage of the total number of particles scored (Table I). In addition, cells from the same experiment were scanned along their apical area to measure the ratio between clathrin-coated pits and clathrin-coated vesicles. This was done directly from the screen of the microscope working at a magnification of 30,000. Only coated structures found on the apical membrane or in the cytoplasm within a distance of 300 nm from the apical membrane (approximately threefold the typical thickness of a coated vesicle) were considered. A total number of 100 coated structures (labeled or not) from fields randomly sampled were scored, and the ratio between pits and vesicles was calculated in normal and MAL-depleted MDCK cells.

Online supplemental material
Video 1 accompanies Fig. 2 and shows two examples of cointernalization of pIgR–antibody complexes (red) and MAL-GFP (green) in MDCK cells. Frames were collected every 5 s. The display rate is 9.5 frames/s. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200304053/DC1.

	Acknowledgments

 
We thank S. Gómez and C. Sánchez for technical help.

This work was supported by grants from the Comunidad de Madrid (08.5/0066/2001.1), Ministerio de Ciencia y Tecnología (PM99-0092 and BMC2003-03297), Fondo de Investigación Sanitaria (01/0085-01), and Fundación Eugenio Rodríguez Pascual to M.A. Alonso; from Ministerio de Ciencia y Tecnología (PM99-0137 and BFI2000-0156) to J. Ballesta; and Fundación Séneca (PB/49/FS/02) to J.A. Martínez-Menárguez. An institutional support from Fundación Ramón Areces is also acknowledged.

Submitted: 10 April 2003

Accepted: 14 August 2003

	References

Top Abstract Introduction Results Discussion Materials and methods References

 

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