The Dendritic Cell Receptor for Endocytosis, Dec-205, Can Recycle and Enhance Antigen Presentation via Major Histocompatibility Complex Class II-Positive Lysosomal Compartments

doi:10.1083/jcb.151.3.673

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Published online 30 October 2000. doi:10.1083/jcb.151.3.673

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© The Rockefeller University Press, 0021-9525/2000//673 $5.00
The Journal of Cell Biology, Volume 151, Number 3, , 2000 673-684

Original Article

The Dendritic Cell Receptor for Endocytosis, Dec-205, Can Recycle and Enhance Antigen Presentation via Major Histocompatibility Complex Class II–Positive Lysosomal Compartments

Karsten Mahnke^a, Ming Guo^b, Sena Lee^b, Homero Sepulveda^c, Suzy L. Swain^c, Michel Nussenzweig^b, and Ralph M. Steinman^a

^a Laboratory of Cellular Physiology and Immunology, The Rockefeller University, New York, New York, 10021
^b Howard Hughes Medical Institute, The Rockefeller University, New York, New York, 10021
^c The Trudeau Institute, Saranac Lake, New York 12983
Laboratory of Cellular Physiology and Immunology, The Rockefeller University, 1230 York Ave., New York, NY, 10021-6399.(212) 327-8875(212) 327-8106

Many receptors for endocytosis recycle into and out of cellsthrough early endosomes. We now find in dendritic cells thatthe DEC-205 multilectin receptor targets late endosomes or lysosomesrich in major histocompatibility complex class II (MHC II) products,whereas the homologous macrophage mannose receptor (MMR), asexpected, is found in more peripheral endosomes. To analyzethis finding, the cytosolic tails of DEC-205 and MMR were fusedto the external domain of the CD16 Fc ${gamma}$ receptor and studied instable L cell transfectants. The two cytosolic domains eachmediated rapid uptake of human immunoglobulin (Ig)G followedby recycling of intact CD16 to the cell surface. However, theDEC-205 tail recycled the CD16 through MHC II–positivelate endosomal/lysosomal vacuoles and also mediated a 100-foldincrease in antigen presentation. The mechanism of late endosomaltargeting, which occurred in the absence of human IgG, involvedtwo functional regions: a membrane-proximal region with a coatedpit sequence for uptake, and a distal region with an EDE triadfor the unusual deeper targeting. Therefore, the DEC-205 cytosolicdomain mediates a new pathway of receptor-mediated endocytosisthat entails efficient recycling through late endosomes anda greatly enhanced efficiency of antigen presentation to CD4⁺T cells.

Key Words: dendritic cell • antigen presentation • DEC-205 • MHC class II • endocytosis

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Several cell surface receptors deliver ligands to the endocyticsystem for purposes of extensive intracellular digestion withinlysosomes. Many of these receptors function exclusively in endocytosis,such as the prototype low-density lipoprotein receptor (LDLR)(Brown et al. 1983) and asialoglycoprotein receptor (Ciechanover et al. 1983).These localize to coated pits, dramatically increasing uptakevia coated vesicles. After ligand release in early endosomes,the receptors recycle rapidly to the cell surface. By avoidingproteolysis during this recycling, such receptors are idealfor nutrient delivery and scavenging, e.g., cholesterol, iron,and altered glycoproteins. Other receptors, e.g., those forimmune complexes (Amigorena et al. 1992a) and certain growthfactors (Wilde et al. 1999), have signaling functions in additionto mediating adsorptive uptake of their ligands. The receptorstypically are catabolized in lysosomes, rather than recycled,after uptake of immune complexes and growth factors (Mellman et al. 1983).This receptor downregulation can dampen signal transduction.The ligands for both recycling and nonrecycling families ofendocytic receptors are digested in lysosomes down to the levelof amino acids. Digestion must be complete, since amino acidsand monosaccharides are then able to diffuse out of the lysosomalsystem. Incomplete digestion, as occurs with lysosomal enzymedeficiency, leads to vacuolar swelling (Cohn and Ehrenreich 1969;Ehrenreich and Cohn 1969).

Adsorptive endocytosis receptors, like the macrophage mannosereceptor (MMR), FcR, and B cell antigen receptor (BCR), areused in the immune system to facilitate antigen capture andpresentation of peptides to T cells (Bonnerot et al. 1992; Sallusto et al. 1995;Engering et al. 1997). Previously we have identified an endocyticreceptor, termed DEC-205, expressed by dendritic cells (DCs).This 205-kD protein contains 10 external, contiguous, C-typelectin domains and by sequence analysis, is a homologue of theMMR. In fact, both the MMR and DEC-205 mediate adsorptive uptake,and both have cytosolic domains with requisite coated pit localizationsequences (Stahl et al. 1980; Jiang et al. 1995). Therefore,we expected that both MMR and DEC-205 would recycle throughearly endosomal compartments and present bound antigens comparably.However, we will show that DEC-205 unexpectedly targets to lateendosomes or lysosomes in developing DCs, and that DEC-205 isfar superior to the MMR in presenting bound rabbit antireceptorantibodies to T cells, a classical assay for measuring the presentingfunction of endocytosis receptors (Chesnut and Grey 1981).

To dissect the role of the cytosolic domain in these findings,we studied a totally heterologous system: L cells stably transfectedwith a fusion receptor formed between the external domains ofhuman CD16 and different cytosolic tails. We find that the DEC-205cytosolic domain has a distinct distal region with an acidicEDE triad. The distal region and its acidic sequence are requiredfor recycling beyond early endosomes through deeper major histocompatibilitycomplex class II–positive (MHC II⁺), late endosomes andlysosomes. Such distal targeting is unique for adsorptive endocytosisreceptors that have been analyzed to date, and proves to benecessary for presentation of antigenic peptides at low dosesof ligand. This new pathway for receptor-mediated uptake istherefore a hybrid of the two known endocytic pathways discussedabove, targeting deeper digestive compartments but recyclingefficiently to produce biologically active peptides.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Cells
The MHC II (I-E^k)–expressing cell line DCEK.ICAM.Hi7 wasmaintained in RPMI with 7.5% Ig-depleted FCS (Atlanta Biologicals),10 IU/ml penicillin/streptomycin, 200 µM/ml glutamine(GIBCO BRL), and 50 µM 2-mercaptoethanol (Sigma-Aldrich)(R7 medium). To maintain MHC II and intracellular adhesion molecule(ICAM)-1 expression, every other week the cells were kept inMXH medium (R7 containing 6 µg/ml mycophenolic acid, 250µg/ml xanthine, 15 µg/ml hypoxanthine [all fromSigma-Aldrich], and 800 µg/ml G418 [GIBCO BRL]). CD16chimeric receptor transfectants were kept in MXH medium additionallysupplemented with 5 µg/ml puromycin (Calbiochem). DCswere generated from mouse bone marrow cultured in the presenceof GM-CSF as described previously (Inaba et al. 1992). Day 6DCs are primarily at an immature, antigen-capturing stage ofdevelopment (Pierre et al. 1997).

Cloning and Transfection
The cDNAs coding for the intracellular domains of DEC-205 andMMR were cloned separately from the extracellular expresseddomains into a TA vector (Invitrogen), and oligonucleotide directedmutagenesis using QuikChange^® (Stratagene) was performed.STOP codons and a tyrosine to alanine exchange were introducedinto different parts of the DEC tail (see Fig. 1 A). All mutationswere verified by sequencing (DNA Technology Center, The RockefellerUniversity). Using standard methods, the mutated DEC tails werecloned into the BamH1-EcoR1 site of the pApuro vector (giftof Dr. Kurosaki, American Cynamid Company, Lederle Laboratories,Department of Cardiovascular Molecular Biology, Pearl River,NY) behind the sequence coding for the extracellular domainof the human Fc ${gamma}$ III receptor (Kolanus et al. 1993). After verifyingthe correct insertion by sequencing, these constructs were transfectedinto the MHC II⁺ (I-E^k) fibroblast cell line DCEK.ICAM.Hi7 bycalcium phosphate precipitation (Stratagene). Thereafter, cellswere split into 100-mm dishes and for selection, puromycin (Calbiochem)was applied at a final concentration of 5 µg/ml. Coloniesgrowing under selection after 2–3 wk were picked and expanded.Surface expression of CD16 was regularly monitored by FACS^®,using anti-CD16 antibody (clone 3G8).

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Figure 1 Distinct intracellular localization and function of DEC-205 and MMR in DCs. (A) Localization. Immature day 6 bone marrow DCs (BmDC) (Inaba et al. 1992) were seeded on coverslips, fixed, and double stained with rabbit anti–DEC-205 and MMR (red), and the late endosomal/lysosomal components, LAMP-1 or MHC II (green). Examples of individual granules that contain red and green label are marked by arrows, and colocalization is further shown in yellow in the merged images. (B) Surface binding and presentation of anti–DEC-205 and MMR antibodies. Day 6, immature marrow-derived DCs were incubated with different dilutions (as indicated) of anti–DEC-205, anti-MMR, or preimmune rabbit serum on ice for 1 h. Unbound antibody was washed away. The cells were incubated with FITC-labeled anti-Ig, to assess amounts of surface bound antibody by FACS^® (top), or cocultured in graded doses with rabbit IgG–primed T cells, to measure presentation of peptides from rabbit antibodies (bottom). (C) DCs were incubated with 1:100 dilution of anti–DEC-205 or anti-MMR rabbit serum on ice for 1 h. Unbound antibody was washed away, and presentation of peptides from rabbit antibodies was assayed by coculturing the DCs with graded doses of T cells primed with anti–DEC-205 or anti-MMR antiserum, respectively.

Flow Cytometric Analysis of Surface Markers
Cells were harvested with trypsin (Boehringer), then incubatedwith cold PBS/7% normal goat serum (vol/vol) followed by incubationfor 45 min on ice with the following hybridoma supernatants:anti–MHC II (14-4-4S; American Type Culture Collection),anti–ICAM-1 (YN-1; American Type Culture Collection),and anti-CD16 (3G8). B7 expression was assayed with anti–B7-1antibody (1G10; BD PharMingen). After washing with cold PBS/1%FCS (vol/vol), FITC-labeled mouse anti–rat Ig or goatanti–mouse Ig (Jackson ImmunoResearch Laboratories) secondaryreagents at a final dilution of 1 µg/ml in PBS/1% FCS(vol/vol) were added. After 45 min on ice, cells were washedand resuspended in PBS containing 1 µM propidium iodide(Sigma-Aldrich) to gate out dead cells during analysis for fluorescenceusing a FACScan^TM (Becton Dickinson).

Surface Binding and Internalization of Human IgG
Human IgG (HuIgG; Jackson ImmunoResearch Laboratories) was dilutedto 1 mg/ml in PBS. Aggregates were formed by incubation at 65°Cfor 30 min. Thereafter, aliquots were stored at 4°C untiluse, but no longer than 1 wk. In some antigen-presenting assays,HuIgG was aggregated by incubation with goat anti-HuIgG antibodiesfor 4 h at room temperature. To assay surface binding of HuIgG,cells were harvested and washed with cold PBS/1% FCS (vol/vol)and incubated for 45 min on ice with monomeric or aggregatedHuIgG (aggHuIgG) at 0.1–100 µg/ml. After washeswith cold PBS/1% FCS (vol/vol), FITC-labeled goat anti–humanIgG antibodies (Jackson ImmunoResearch Laboratories) at a finalconcentration of 1 µg/ml in PBS/1% FCS (vol/vol) wereadded. After 45 min on ice, cells were washed, resuspended inPBS, and analyzed on a FACScan^TM. To measure internalized HuIgG,the DCEK.ICAM.Hi7 cells were seeded into 96-well plates (20,000cells/well), cultured overnight, and transferred on ice followedby addition of HuIgG at a final concentration of 50 µg/ml.After 45 min, unbound HuIgG was removed by washing with medium,and aliquots of cells were harvested and fixed with 4% paraformaldehyde(PFA). The remaining cells were further incubated in R7 at 37°Cafter which the cells were harvested, fixed, and stained withFITC-labeled goat anti–human IgG antibodies as describedabove. To detect internalized HuIgG, cells were permeabilizedbefore adding FITC-labeled goat anti–human antibodies,using a 10-min incubation with PBS/0.1% (vol/wt) saponin (Sigma-Aldrich).In time course experiments, the amount of internalized HuIgGwas calculated by subtracting the mean fluorescence in fixedcells (surface-bound HuIgG) from that recorded with fixed andpermeabilized cells (internalized and surface-bound HuIgG).

Receptor Recycling
Cells were cultured for 2 h in 10 µg/ml cycloheximide(CHX; Calbiochem), sufficient to block protein biosynthesisas assessed by [³⁵S]methionine labeling (not shown). SurfaceCD16 then was saturated by incubating the cells in presenceof CXH with aggHuIgG (100 µg/ml) at 37°C for 10 min,followed by chilling the cells for 1 h on ice. Thereafter, cellswere cultivated in R7 supplemented with CXH, and at differenttimes, recycled CD16 receptors were detected by incubation with¹²⁵I-HuIgG at 10 µg/ml on ice. Bound HuIgG was measuredby ${gamma}$ counting (Wallac).

Confocal Immunofluorescence Microscopy of L Cells and DCs
L cells were seeded into LabTek tissue culture chambers (Nunc)and incubated overnight. Cells were washed twice with warm RPMImedium, fixed with 4% paraformaldehyde/PBS (wt/vol) for 20 minat room temperature, and permeabilized by incubation with permeabilizationbuffer (RPMI containing 10% normal goat serum [GIBCO BRL], 0.05%saponin [Sigma-Aldrich], 10 mM glycine [Sigma-Aldrich]) for15 min at room temperature. Alternatively, DCs were grown frombone marrow precursors using GM-CSF as described (Inaba et al. 1992).At day 6, when the cultures contain numerous aggregates of immatureDCs with abundant MHC II compartments (MIICs) (Pierre et al. 1997),the cells were dislodged and applied to alcian blue–coated,glass slides for fixation as above. After two washes in permeabilizationbuffer, cells were incubated for 45 min at room temperaturewith the following antibodies: anti–MHC II (M5/114; AmericanType Culture Collection), anti–lysosome-associated membraneprotein 1 (LAMP-1) (clone ID-4B; gift of Dr. Ira Mellman, YaleUniversity School of Medicine, New Haven, CT), anti-transferrinreceptor (TfR) (C2F2; American Type Culture Collection), anti-CD16(clone 3G8), and either monoclonal or polyclonal antibody toDEC-205 (Swiggard et al. 1995) and MMR (prepared in rabbitsby immunization with cloned MMR external domains). In doublelabeling experiments, FITC-conjugated MHC II and LAMP-1 antibodies(BD PharMingen) were used. For unconjugated antibodies, we stainedcells for 45 min in permeabilization buffer with appropriateFITC- or Texas red–labeled secondary reagents, absorbedagainst mouse or rat proteins and applied at a final concentrationof 1 µg/ml. For detection of endocytosed HuIgG, FITC-labeledgoat anti-HuIgG was applied at 1 µg/ml in permeabilizationbuffer. Slides were mounted in aquamount (Polysciences) andexamined by confocal laser scan microscopy (ZEISS). ZEISS softwarewas used to take and to overlay pictures. Composite figureswere made using Photoshop^® (Adobe Systems).

Antigen Presentation to T Cells
To obtain HuIgG- or RbIgG-specific T cells, 6–8-wk-oldB10.BR mice (The Jackson Laboratory) were primed to HuIgG orRbIgG by subcutaneous injection of 50 µg HuIgG or RbIgGemulsified in complete Freund's adjuvant (Difco). In some experiments,mice were primed to RbIgG using anti–DEC-205 Rb antiserumor anti-MMR Rb antiserum. 8 d later, draining lymph nodes wereremoved and single cell suspensions were prepared by teasingwith forceps and forcing the nodes through a nylon mesh. T cellswere purified by passage over nylon wool columns and incubatingthe eluted cells with antibodies directed against MHC II (M5/114;American Type Culture Collection) and CD45 (B220; American TypeCulture Collection) on ice for 30 min. In some experiments,anti-CD8 antibodies (TIB 211; American Type Culture Collection)were added to obtain purified CD4⁺ T cells. Cells were washedand incubated with goat anti–rat Dynabeads (Dynal) ata ratio of 4 beads to 1 target cell for an additional 30 minat 4°C to remove non-T cells. For antigen presentation assayswith DCEK.ICAM.Hi7 cells, transfected and untransfected DCEK.ICAM.Hi7cells were irradiated with 5,000 rads and seeded into 96-wellplates (15,000 cells/well). HuIgG was added to the cells ingraded doses. After overnight culture, unbound HuIgG was removedby washing the plates with warm R7 medium. Thereafter, 250,000T cells/well in 200 µl R7 were added in triplicate, andthe plates were incubated for 3–4 d. For antigen presentationassays with DCs, developing bone marrow DCs were harvested after6 d of culture in GM-CSF, placed on ice, and incubated withgraded doses of rabbit anti–DEC-205, anti-MMR, and preimmuneserum for 1 h. Unbound antibodies were washed away and aliquotsof the DCs were seeded in triplicates into 96-well plates. Then200,000 T cells/well were added and cultured for 3–4 d.To assay T cell proliferation, [³H]thymidine (1 µCi/well;Amersham Pharmacia Biotech) was added for the last 12 h beforeharvesting. Incorporation of radioactivity was determined byscintillation counting. Data are shown are means of triplicateswhere the standard deviation was <10% of the mean cpm.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Unique Localization and Function of DEC-205 in DCs
DEC-205 belongs to the group VI family of lectins (Drickamer and Taylor 1993)that contain 8–10 extracellular, contiguous C-type lectindomains and include the MMR. Both DEC-205 and MMR can be expressedon DCs (Jiang et al. 1995; Engering et al. 1997). Rabbit polyclonalantibodies to mouse DEC-205 (Swiggard et al. 1995) and the mouseMMR (our unpublished data) were used to localize these receptorsin developing mouse DCs, generated from bone marrow progenitorswith GM-CSF (Inaba et al. 1992). By day 6, the cultures werepredominantly immature DCs with endocytic activity and abundant,intracellular, late endosomes or lysosomes (Pierre et al. 1997).These compartments were rich in MHC II products and are calledMIICs.

By confocal laser scan microscopy, both the MMR and DEC-205were abundant in intracellular granules (Fig. 1 A, red). Asexpected for a recycling endocytic receptor, very little ofthe MMR was found in late endosomes or lysosomes that were labeledfor LAMP-1 or for MHC II (Fig. 1 A, green and merge images).In marked contrast, the bulk of the intracellular DEC-205 waslocalized in perinuclear MIICs, as demonstrated by colocalizationwith LAMP-1 and with MHC II (Fig. 1 A).

To detect a functional consequence for the distinct targetingof the MMR and DEC-205, we used the rabbit polyclonal antibodiesas surrogate antigens for T cells primed to rabbit Ig, as Chesnut and Grey 1981first did to show presentation via the BCR. When antibodieswere added to immature DCs in the cold, the cells bound comparableamounts of anti-MMR and DEC-205 Ig (Fig. 1 B, top). When thesame cells were added to cultures of primed T cells, the anti–DEC-205was presented with much higher efficiency (Fig. 1 B, bottom).To rule out that the quantitative difference is due to differentallotypic determinants within the MMR and DEC-205 antibodies,additional experiments were performed using T cells from miceprimed to RbIgG with either anti–DEC-205 or anti-MMR antiserum(Fig. 1 C). Here again the anti–DEC-205 was presentedwith much higher efficiency regardless of whether the T cellswere derived from animals primed with either DEC-205 or MMRantibodies. Thus, DEC-205 is normally found in MIICs, whereasMMR is predominantly found in early endosomes; when rabbit antibodiesare bound to these two receptors, DEC-205 is much more efficientat presenting peptides to rabbit Ig–primed, CD4⁺ T cells.

Expression of Chimeric DEC-205/CD16 Receptors in Transfected DCEK.ICAM.Hi7 Cells
The targeting of endocytic receptors is determined by aminoacid sequences within their intracellular domains (for reviewsee Bonifacino and Dell'Angelica 1999). A reexamination of thecytosolic domains ("tails") of three homologous lectins—theMMR, DEC-205, and the phospholipase A2 receptor (PLA2R)—showedthe tails of the MMR and PLA2R to be very similar to each otherbut different from DEC-205 (gray shading in Fig. 2 A). All threetails contained a membrane-proximal, putative coated pit localizationsequence (Fig. 2 A, underlined) for uptake (Collawn et al. 1990),but the distal region of DEC-205 was distinct and included asequence of three acidic amino acids (Fig. 2 A, EDE). Interestingly,acidic sequences in other receptors are implicated in intracellularsorting (Matter et al. 1993; Voorhees et al. 1995; Wan et al. 1998;Piguet et al. 1999; Simmen et al. 1999).

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Figure 2 Cytosolic domains used to study the targeting of endocytosis receptors. (A) Sequences of the cytoplasmic domain of three multilectin receptors for adsorptive endocytosis: DEC-205, PLA2R, and MMR. Underlining indicates a consensus sequence for endocytosis via coated pits; boldface indicates a cluster of acidic residues (EDE), postulated to guide DEC-205 beyond early endosomes; gray shading shows similar amino acids in the tails. (B) Mutations were introduced into the DEC tail (arrows), leading to truncations at the sites denoted (ST, short tail; IT, intermediate tail; LT, long tail), or to amino acid substitutions: Y to A in alternate tail (AT), and EDE to AAA in the AAA tail. (C) Surface expression of CD16 and MHC II in untransfected DCEK.ICAM.Hi7 cells (none) or cells transfected with CD16 fusion receptors (WT, LT, IT, ST, AT, AAA, and MMR). Staining was with anti-CD16 (clone 3G8), anti–I-E^k (clone HB32), or isotype control anti–I-A^k (clone 10.216), followed by FITC goat anti–mouse F(ab')₂ antibodies.

To determine which components of the cytoplasmic tail were requiredfor efficient targeting and presentation via late endosomesor lysosomes (Fig. 1), we constructed chimeric receptors containingthe external IgG binding domain of the HuFc ${gamma}$ III receptor or CD16and different DEC-205 cytosolic tails (Fig. 2 B). In additionto the wild-type (WT) DEC-205 tail, we made truncations to removethe terminal three amino acids (long tail, LT), residues 19–31with the putative EDE distal targeting sequence (intermediatetail, IT), and residues 6–31 with the coated pit sequence(short tail, ST). We also made mutants of the DEC-205 tail,converting tyrosine to alanine in the coated pit sequence (alteredtail or AT), and EDE to alanines in the putative distal targetingsequence. We used the wild-type MMR tail for comparison.

The CD16 chimeras were transfected into a murine fibroblast-likeline, DCEK.ICAM.Hi7, which expresses MHC II as well as the Tcell costimulatory molecules B7-1 (CD80) and ICAM-1 (CD54) (Dubey et al. 1995).Comparable surface expression of each CD16 chimeric receptorwas obtained (Fig. 2 C) in the stable transfectants, withoutaltering expression of MHC II (Fig. 2 C) or B7-1 (not shown).

Binding, Uptake, and Recycling of HuIgG by CD16 Chimeric Receptors
To test the function of the chimeric receptors, we first measuredbinding of HuIgG as illustrated for WT-DEC:CD16 (Fig. 3 A).The transfectants all bound ligand. Saturation occurred at 10µg/ml, whereas the untransfected DCEK.ICAM.Hi7 cell line(Fig. 3 A, none) did not bind HuIgG. Binding required that thehuman IgG be heat aggregated, as expected for functional Fc ${gamma}$ RIII(Unkeless et al. 1981). On PAGE, <10% of the HuIgG aggregated(molecular mass > 200,000 D) upon heating to 65°C for30 min (Fig. 3 B), so that saturable binding of the expressedchimeric receptors was occurring at <1 µg/ml of aggHuIgG.When the sensitivity of bound ligand to pH was measured, aggHuIgGbegan to elute at pH 5, and only 40% remained at pH 4 (Fig. 3C).

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Figure 3 Ligand binding, uptake, and recycling via CD16 DEC-205 chimeric receptors. (A) Binding of aggHuIgG to transfected cells. WT-DEC/CD16 transfected cells (WT) and untransfected cells (None) were incubated on ice for 1 h with graded doses of aggHuIgG. After washing, surface-bound IgG was detected with FITC goat anti-HuIgG F(ab')₂ and FACS^®. Cells were also stained for surface CD16 using 3G8 and FITC goat anti–mouse F(ab')₂. Binding to WT cells and all other transfectants (see Fig. 1) was similar. (B) To detect the small amount of aggHuIgG in the heated HuIgG preparations, samples were analyzed under reducing conditions by SDS-PAGE analysis. (C) Elution of HuIgG to CD16 at acidic pH. Elution of aggHuIgG to CD16 was performed at different pH's, predicting a release of ligand in mildly acidic compartments. (D) Endocytosis of aggHuIgG. Untransfected cells (none) and transfectants with different DEC:CD16 chimeric receptors (WT, ST) were incubated on ice for 1 h with aggHuIgG (10 µg/ml). Aliquots were fixed and stained for surface-bound HuIgG immediately (bold line) or incubated at 37°C for 4 h (thin line) before fixation and staining with FITC-labeled anti-HuIgG (first column, fixed only). Cells were also permeabilized before staining with FITC-labeled anti-HuIgG (second column) to reveal endocytosed HuIgG. (E) Uptake of HuIgG. Cell lines were incubated with aggHuIgG on ice, transferred to 37°C for different times, and stained with FITC-labeled anti-HuIgG F(ab')₂ without or with prior permeabilization. The mean fluorescence was determined by FACS^® analysis, and the amount of internalized IgG was plotted as a percentage of total surface-bound IgG. (F) Recycling of CD16 chimeric receptors. Cells were treated for 2 h with CHX and then incubated with 100 µg/ml aggHuIgG, and transferred on ice, to saturate binding of all CD16 chimeric receptors (see Fig. 2 A). After washing, the cells were incubated at 37°C in the continued presence of CHX for different times, and recycling CD16 chimeric receptors were detected by binding of ¹²⁵I-HuIgG. The amount of recycled receptors is plotted as a percentage of the amount of surface-bound ¹²⁵I-HuIgG obtained with untreated cells.

To monitor endocytosis, aggHuIgG was bound to each transfectanton ice, and aliquots were transferred to 37°C for 2 h. TheFACS^® was used to follow uptake at the single cell level.Binding of FITC anti-HuIgG to fixed cells detected residualsurface HuIgG, and to fixed permeabilized cells, detected surfaceand intracellular HuIgG. With WT-DEC:CD16–expressing cells,HuIgG was no longer detectable at the surface after the 2-hchase at 37°C (Fig. 3 D), but strong staining was obtainedin permeabilized cells, indicating that the DEC tail mediateduptake of ligands bound to a heterologous receptor.

Similar results, i.e., endocytosis of bound HuIgG, were obtainedwith cells expressing the LT-, IT-, and AT-DEC:CD16 chimera(not shown). In contrast, cells transfected with the short six–aminoacid tail (ST-DEC:CD16), lacking the putative coated pit localizationsequence, showed no significant loss of surface IgG (Fig. 3D), indicating that deletion of amino acid residues 6–31prevents endocytosis of the DEC:CD16 chimeric receptor. In amore detailed time course study (Fig. 3 E), we included cellsexpressing AAA-DEC:CD16 and MMR:CD16. Again, the ST-DEC:CD16chimera did not internalize, whereas half the surface Ig enteredthe cells via the other CD16 chimeras within 15 min. The AT-DEC:CD16chimera, which contained a mutation of the tyrosine residuein the coated pit localization site, was capable of endocytosisalthough at a somewhat slower rate (Fig. 3 E). Therefore, allthe chimeric CD16 receptors bound aggHuIgG, and all except theST-DEC:CD16 mediated rapid adsorptive uptake of ligand.

To examine recycling of the DEC:CD16 chimeric receptors, weblocked protein synthesis using CHX at 10 µg/ml for 2h. We then added a saturating dose of aggHuIgG, placed the cellson ice, washed, and transferred the L cells to 37°C. Thisprocedure was sufficient to saturate all of the CD16 chimericreceptors (data not shown). Thereafter, at subsequent time points,we added ¹²⁵I-labeled aggHuIgG to detect a reappearance of functionalCD16 receptors. The intact cytosolic tails (WT, MMR) recycledwithin 1 h after internalization, but the truncated intermediateDEC tail (IT) and the AAA-DEC:CD16 chimera recycled less rapidly(Fig. 3 F). The 1-h recycling time could underestimate the speedof recycling via the DEC-205 tail, because the pH of the vacuolarsystem in L cells may be insufficiently low to quickly eluteall of the bound HuIgG ligand. As expected, the ST tail didnot recycle, i.e., regenerate functional CD16, because endocytosiswas not occurring. To rule out replenishment of receptors fromendocytic pools, rather than recycling, we repeated the experimentsin cells exposed for 1 h at 37°C to aggHuIgG to occupy intracellularstores. Again, recycling of new HuIgG binding receptors tookplace (data not shown). We conclude that the DEC-205 and MMRtails are each capable of mediating ligand uptake, discharge,and recycling to the cell surface, and that these activitiescan be carried out by all of the mutant cytosolic tails we hadprepared, except for the short tail lacking the coated pit localizationand uptake sequence.

Intracellular Compartments Targeted by CD16 Chimeric Receptors
At this stage of the studies, the DEC-205 and MMR tails seemedsimilar. Distinctive features of the DEC-205 tail became apparentupon examining the intracellular targeting of CD16 chimericreceptors and HuIgG ligand, and in tests of antigen presentationto HuIgG-primed T cells. First, we did confocal immunofluorescencemicroscopy to simultaneously identify MHC II and LAMP-1 or theearly endosomal marker TfR. In all transfectants (WT shown here),MHC II largely colocalized with LAMP-1, a marker for late endosomes/lysosomesin the perinuclear region (Fig. 4, top), and not with TfR inthe periphery (Fig. 4, bottom).

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Figure 4 Presence of MHC II⁺ lysosomal compartments in CD16 transfectants (WT-DEC:CD16 shown here). Stably transfected DCEK.ICAM.Hi7 cells on tissue culture chamber slides were fixed and double labeled for MHC II and lysosomal (LAMP-1) proteins (top) or TfR (bottom). Primary antibodies were visualized by FITC- and Texas red–labeled secondary antibodies. By confocal laser scan microscopy, MHC II colocalizes with LAMP-1 in all cells (yellow) but not with the TfR.

In either the absence or presence of IgG ligand, WT-DEC:CD16chimeric receptors efficiently localized to late endosomal/lysosomalcompartments, as shown by colocalization with LAMP-1 and MHCII in the perinuclear region (left columns of Fig. 5A and Fig. B,respectively). In contrast, the MMR:CD16 did not colocalizewith LAMP-1 and was found primarily in the peripheral cytoplasm(Fig. 5 A). Receptor targeting to late endosomes was mediatedby sequences found in the distal portion of the cytoplasmictail of DEC-205, since DEC-IT:CD16 chimeras, which lacked aminoacids 18–31 in the cytoplasmic tail of DEC-205, failedto accumulate in MHC II⁺ lysosomes and were found in vesiclesthroughout the cytoplasm (Fig. 5A and Fig. B). The ST-DEC:CD16chimera failed to mediate endocytosis completely, and was distributedalong the cell membrane (Fig. 5 A).

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Figure 5 Typical distribution of CD16 chimeric receptors in DCEK.ICAM.Hi7 cells in the absence (shown here) or presence of ligand, 10 µg/ml aggHuIgG. (A) CD16 and LAMP-1 double labeling. Cells on tissue culture chamber slides were fixed and stained for CD16 (green, FITC-labeled anti–mouse Ig) and LAMP-1 (red, Texas red–labeled anti–rat Ig). Colocalization in discrete vesicles in WT transfected cells is indicated by arrows, and for all the transfectants is displayed in yellow (bottom row). (B) CD16 and MHC II double labeling. Cells grown on tissue chamber slides were fixed and stained for CD16 (red) or MHC II (green) with species-specific secondary reagents. Slides were analyzed by confocal laser scan microscopy. Examples of colocalization in single vesicles in WT transfected cells are indicated by arrows and displayed in yellow (bottom row).

To follow the targeting of bound ligand, we incubated the Lcells with aggHuIgG for 30 min on ice, followed by a 30-minchase at 37°C. Surface-bound HuIgG was found on all transfectantsafter incubation on ice (Fig. 6 A, top), confirming the FACS^®data (Fig. 3 A). After incubation at 37°C, HuIgG was mainlyfound in lysosomes in WT-DEC:CD16 transfectants, colocalizingwith LAMP-1 in the perinuclear region (Fig. 6 A, bottom left).In contrast, HuIgG endocytosed by either IT-DEC:CD16 or MMR:CD16transfected cells, colocalized with TfR in early endosomes (datanot shown), indicating that ligands bound to these receptorsfailed to reach lysosomes efficiently (Fig. 6). HuIgG boundto the ST-DEC:CD16 chimera remained surface bound during the30-min chase period. From these results, we conclude that theDEC-205 cytoplasmic domain targets CD16 chimeras and their ligandsto MHC II⁺LAMP-1⁺ vacuoles, whereas the cytoplasmic domain ofthe MMR targets primarily to early endosomes. Sequences fortargeting to late endosomes lie between positions 18 and 31in the DEC-205 tail. The different targeting routes of MMR:CD16and AAA-DEC:CD16 versus WT-DEC:CD16 should be reflected in adifferent time course for their recycling of these receptors,but in fact unoccupied receptors reappeared with a similar pace.However, the speed of recycling via early endosomal compartmentsis likely to have been underestimated because the pH of theearly endosomes may be insufficiently low to quickly elute allof the bound HuIgG ligand.

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Figure 6 Intracellular localization of endocytosed HuIgG in CD16 transfectants. (A) Double labeling for endocytosed HuIgG and LAMP-1. Cells, grown on tissue chamber slides, were incubated with 10 µg/ml HuIgG for 1 h on ice. Unbound HuIgG was washed away and cells were either fixed immediately or further incubated in medium for 30 min at 37°C. Cells were double stained with FITC-labeled anti-HuIgG (green) and with anti–LAMP-1 antibodies (red; Texas red–labeled secondary antibodies).

Presentation of Ligands Internalized by Chimeric CD16 Receptors to CD4⁺ T Cells
To determine whether antigen bound to CD16 chimeric receptorswas processed and presented, we pulsed the transfected cellswith aggHuIgG for 6 h, and assayed for presentation to primedT lymphocytes. Cells expressing WT-DEC:CD16 induced strong Tcell proliferation, with saturation concentrations of 1 µg/mlaggHuIgG (Fig. 7 A). Immune complexes formed with anti-HuIgGand soluble HuIgG were also presented efficiently, whereas nonaggregatedHuIgG, which did not bind to CD16 receptors (Fig. 3 A), onlyinduced occasional T cell proliferation at high doses (100 µg/ml;Fig. 7B and Fig. C).

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Figure 7 Antigen presentation by DEC-CD16 transfected cells. (A) Presentation of aggHuIgG. Transfected and untransfected (none) DCEK.ICAM.Hi7 cell lines were incubated for 6 h with aggHuIgG, washed, and used to present antigen to 250,000 purified lymph node T cells from mice primed to HuIgG. At 72 h, the cells were pulsed with [³H]thymidine for 12 h, and incorporated radioactivity was measured. (B) Presentation of immune complexes of HuIgG. As in A, transfected and untransfected (none) DCEK.ICAM.Hi7 cell lines were incubated with either soluble or antibody aggregated HuIgG. Antigen presenting assays were then performed.

When the mutant cytosolic tails were studied, LT-DEC:CD16 chimeraswere indistinguishable from WT-DEC:CD16 in inducing T cell proliferationat low antigen concentrations. AT-DEC:CD16 chimeras (tyrosine15 substituted by alanine) showed only a slightly diminishedresponse. In contrast, IT-DEC:CD16, which mediated endocytosisand recycling (Fig. 3E and Fig. F) but failed to target to MHCII⁺LAMP-1⁺ compartments (Fig. 5), was inefficient for antigenpresentation. Cells expressing MMR:CD16 chimeras resembled thoseexpressing IT-DEC:CD16 in that they were only able to stimulateT cell proliferation at high concentrations of HuIgG (10–100µg/ml; Fig. 7). ST-DEC:CD16 (lacking the 25 most distalamino acids in the DEC-205 cytoplasmic domain) did not stimulateT cell proliferation above the background obtained with untransfectedDCEK.ICAM.Hi7 cells. These data indicate that sequences requiredto target antigens for efficient presentation differ from thoserequired for endocytosis and recycling. IT-DEC:CD16 and MMR:CD16chimeras mediate endocytosis and recycling, but additional informationfound between amino acids 18 and 28 in the DEC-205 cytoplasmicdomain is required for targeting to antigen processing compartments.

Importance of the Distal EDE Sequence in the Distinct Targeting of the DEC-205 Tail
Acidic amino acids are implicated in intracellular targeting,e.g., the movement of HIV-1 nef protein to lysosomes (Piguet et al. 1999),the movement of furin to the trans-Golgi network (Voorhees et al. 1995;Simmen et al. 1999), and the retrieval of the LDLR from apicalto basolateral membranes of epithelial cells (Matter et al. 1993).To assess if acidic amino acids in the distal part of the DEC-205tail were required for late endosomal targeting, we mutatedthe EDE residues to alanines (AAA-DEC:CD16). The AAA-DEC:CD16chimera was fully competent for adsorptive uptake of aggHuIgGand recycling back to the surface (Fig. 3E and Fig. F), butfailed to target aggHuIgG or CD16 to lysosomes (Fig. 5 B). Consistentwith the absence of late endosomal targeting, presentation ofantigen to IgG-primed T cells was greatly reduced (Fig. 7 A)and occurred only at antigen levels comparable to those neededfor IT-DEC:CD16– and MMR:CD16-mediated presentation. Thus,the EDE in the DEC-205 tail is required for its unique lysosomaltargeting and antigen presenting functions.

Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

A Specialized Receptor for Antigen Uptake and Presentation on DCs
High doses of protein antigens, e.g., 100–1,000 µg/ml,are typically added to antigen-presenting cells to generatethe MHC II–peptide complexes that are ligands for CD4⁺T cells. The efficiency of antigen binding and uptake is greatlyenhanced by receptor-mediated endocytosis, as occurs with theMMR (Engering et al. 1997; Prigozy et al. 1997; Tan et al. 1997),FcR (Sallusto and Lanzavecchia 1994), and BCR (Bonnerot and Lankar 1995).The DEC-205 receptor is expressed by DCs and is a homologueto the MMR, localizing to coated pits and enhancing ligand uptake(Jiang et al. 1995). The MMR primarily recycles through peripheral,early endosomes (Engering et al. 1997; Tan et al. 1997), althoughsome entry into late endosomes is reported (Prigozy et al. 1997).In contrast to the MMR, DEC-205 targets to deep endosomes orlysosomes in DCs rather than early endosomes, the latter beingtypical for other endocytosis receptors. The MMR presents mannosylatedBSA very efficiently (Sallusto et al. 1995). Surprisingly, whenwe used polyclonal rabbit antibodies as surrogate ligands, DEC-205was much more efficient than the MMR in presenting peptidesto rabbit Ig–primed T cells. Since cytosolic domains guidethe movements of adsorptive endocytosis receptors, we proceededto study fusion receptors formed by the external domains ofhuman CD16 and different tails, especially the MMR and DEC-205.In a totally heterologous system, i.e., transfected L cells,the DEC-205 tail mediated a unique recycling pathway throughlate endosomes rich in MHC II, and importantly, greatly enhancedantigen presentation relative to the MMR tail. Typically, Lcells are inefficient at producing MHC II–peptide complexesfrom proteins, and preprocessed peptides are used to study antigenpresentation (Dubey et al. 1995).

Additional work will be needed to pursue the physiological implicationof these findings, i.e., that DEC-205 is used by DCs to improveantigen presentation. The following types of future experimentswould be of value. First, to assess the role of the distal cytoplasmictail in the context of a full length receptor, it would be importantto mutate full length DEC-205; currently, it is not yet feasibleto obtain high level expression of this large receptor. Second,the studies of CD16-DEC fusion receptors could be extended intoDCs using different vectors, and such experiments are underway.Third, ligands for DEC-205 and MMR need to be identified, sothat the presentation of natural ligands rather than surrogatescan be tested. Interestingly, DEC-205 and not the MMR is readilydetected on DCs within the T cell areas of mouse and human lymphoidtissues (Linehan et al. 1999; Guo et al. 2000).

Two Functional Regions of the DEC-205 Cytosolic Domain
The membrane-proximal region of the DEC-205 tail contains thesequence FSSVRY, which resembles the coated pit localizationsequences described in many other receptors (Goldstein et al. 1979).Such sequences function in uptake of the LDLR (Chen et al. 1990;Matter et al. 1993), TfR (Collawn et al. 1990), and MMR (Ezekowitz et al. 1990).The DEC-205 tail is 31 residues in length. Deletion of residues19–31 did not reduce endocytosis, but further deletionof residues 7–19 including the coated pit sequence ablateduptake. Mutation of the tyrosine residue to alanine did notabolish function, in contrast to decreased function of otherreceptors (Chen et al. 1990; Amigorena et al. 1992b; Jackman et al. 1998),but the uptake rates were lower relative to wild-type DEC-205tail. Either the coated pit sequence of DEC-205 is not totallydependent on this tyrosine, or another sequence bypasses itsneed, e.g., the three acidic residues in the distal tail tobe discussed next (Voorhees et al. 1995; Simmen et al. 1999).

The more intriguing region of the DEC-205 cytosolic tail wasthe distal region. Residues 28–31 seemed superfluous,but residues 18–27 were critical for several functions.In the absence of this "distal targeting sequence," the DEC-205tail did not target either receptor or ligand to late endosomesand lysosomes (Fig. 5) and did not mediate efficient antigenpresentation (Fig. 7). However, the distal targeting sequencewas not required for uptake (Fig. 3 E) and membrane recycling(Fig. 3 F).

A cluster of acidic amino acids (EDE) in the distal DEC-205tail proved critical for its distinct intracellular movements(Fig. 5 and Fig. 7). Acidic clusters also mediate trans-Golginetwork retrieval of the mannose-6-phosphate receptor and furin,the latter interacting with a cytosolic sorting molecule PACS-1(Voorhees et al. 1995; Wan et al. 1998; Simmen et al. 1999).Only two acidic amino acids in the HIV-1 nef protein signallysosomal targeting and degradation of endocytosed CD4 moleculesvia β-COP (Piguet et al. 1999). Acidic residues targetthe LDLR to a basolateral site during transcytosis (Matter et al. 1992).The LDLR-related protein contains a cluster of acidic aminoacids as well. This receptor mediates uptake and degradationof sphingolipids, ${alpha}$ 2-macroglobulin, and complement componentC3 into lysosomes (Hiesberger et al. 1998; Meilinger et al. 1999),but the involvement of acidic amino acids in lysosomal targetinghas not been described. The experiments in this paper have comparedDEC-205 with MMR, because of similarities in their externalmultilectin domains and their proposed function in antigen presentation.Future work will compare the cytosolic domains of DEC-205 withthe LDLR family, as well as function in non–antigen-presentingcells like epithelial cells.

A Novel Pathway for an Adsorptive Endocytosis Receptor
As mentioned above (see Introduction), some receptors mediateligand uptake and discharge in early endosomes, followed byrecycling of intact receptors to the surface and further roundsof uptake. Other receptors signal cell activation and growth,and then uptake is followed by ligand and receptor digestionin lysosomes. The new pathway, illustrated by DEC-205, is ahybrid between these two. The cytosolic domain of this receptorcan mediate uptake into deeper vacuoles, followed by recyclingof ostensibly intact receptor. Concomitantly, there is a markedimprovement in the efficiency with which peptides are salvagedand displayed as MHC–peptide complexes. It will be importantnow to follow the distribution and function of DEC-205 in epitheliaand brain endothelium, where this receptor is also abundant.It is possible that in epithelia, as in antigen-presenting cells,DEC-205 will target to deeper proteolytic vacuoles and leadto the production of biologically active peptides.

Acknowledgments

We thank the many colleagues who gave us valuable advice duringpreparation of the manuscript.

These experiments were supported by a fellowship from the DeutscheForschungsgemeinschaft to K. Mahnke (MA 1924/1-1), grants toR.M. Steinman from the Juvenile Diabetes Foundation and theNational Institutes of Health (AI13013 and AI39672), to M. Nussenzweigfrom the Human Science Frontiers Program, and to S. Lee (NationalInstitutes of Health Medical Scientist Training Program grantGM07739).

Submitted: 11 July 2000

Revised: 15 September 2000

Accepted: 15 September 2000

Abbreviations used in this paper: aggHuIgG, aggregated humanIgG; BCR, B cell antigen receptor; CHX, cycloheximide; DC, dendriticcell; ICAM, intracellular adhesion molecule; LAMP-1, lysosome-associatedmembrane protein 1; LDLR, low-density lipoprotein receptor;MMR, macrophage mannose receptor; MHC II, major histocompatibilitycomplex class II; MIIC, MHC II compartment; PLA2R, phospholipaseA2 receptor; TfR, transferrin receptor.

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