Enlargeosome, an Exocytic Vesicle Resistant to Nonionic Detergents, Undergoes Endocytosis via a Nonacidic Route

Emanuele Cocucci^*, Gabriella Racchetti^*, Paola Podini^*, Marjan Rupnik, and Jacopo Meldolesi^*

^* Vita-Salute University, and San Raffaele Scientific Institute, Excellence Center in Cell Differentiation Pathophysiology, 20132 Milan, Italy; European Neuroscience Institute Goettingen, 37073 Goettingen, Germany; and Department of Pharmacology, University of Milan, 20133 Milan, Italy

Submitted July 9, 2004; Revised September 24, 2004; Accepted September 27, 2004
Monitoring Editor: Randy Schekman

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Enlargeosomes, a new type of widely expressed cytoplasmic vesicles,undergo tetanus toxin-insensitive exocytosis in response tocytosolic Ca²⁺ concentration ([Ca²⁺]_i) rises. Cell biology ofenlargeosomes is still largely unknown. By combining immunocytochemistry(marker desmoyokin-Ahnak, d/A) to capacitance electrophysiologyin the enlargeosome-rich, neurosecretion-defective clone PC12-27,we show that 1) the two responses, cell surface enlargementand d/A surface appearance, occur with similar kinetics andin the same low micromolar [Ca²⁺]_i range, no matter whetherinduced by photolysis of the caged Ca²⁺ compound o-nitrophenylEGTA or by the Ca²⁺ ionophore ionomycin. Thus, enlargeosomesseem to account, at least in large part, for the exocytic processestriggered by the two stimulations. 2. The enlargeosome membranesare resistant to nonionic detergents but distinct from otherresistant membranes, rich in caveolin, Thy1, and/or flotillin1.3. Cell cholesterol depletion, which affects many membrane fusions,neither disrupts enlargeosomes nor affects their regulated exocytosis.4. The postexocytic cell surface decline is [Ca²⁺]_i dependent.5. Exocytized d/A-rich membranes are endocytized and traffickedalong an intracellular pathway by nonacidic organelles, distinctfrom classical endosomes and lysosomes. Our data define specificaspects of enlargeosomes and suggest their participation, inaddition to cell differentiation and repair, for which evidencealready exists, to other physiological and pathological processes.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Regulated exocytosis is commonly envisaged as the final stepof regulated secretion, i.e., the stimulation-induced fusionwith the plasmalemma of the membrane of secretory granules andvesicles, followed by the release of their segregated content(for reviews, see Gerber and Sudhof, 2002; Burgoyne and Morgan,2003). Regulated exocytoses, however, are not always secretory.The ultimate task of many of them is in fact the transfer ofmembrane patches, or of their components, from a cytoplasmiccompartment to the cell surface. Processes of this type arewidespread among cells.

Many exocytic, nonsecretory membrane transfers were first revealedby observations documenting the stimulation-induced appearanceat the cell surface of specific integral membrane proteins (Shengand Lee, 2001; Bryant et al., 2002; Brown, 2003). In contrast,in two fibroblast lines (Chinese hamster ovary [CHO] and 3T3;Coorssen et al., 1996; Ninomiya et al., 1996) and in PC12-27(Kasai et al., 1999), a neurosecretory clone defective of regulatedsecretion (Malosio et al., 1999; Grundschober et al., 2002),the first observations, made by electrophysiological capacitance/patchclampassays, consisted in considerable (15–30%) expansionsof the plasma membrane in response to large increases of thecytosolic Ca²⁺ concentration ([Ca²⁺]_i), induced by photolysisof caged Ca²⁺ compounds. In PC12-27, these responses start afew hundreds of milliseconds after stimulation and develop rapidly(t_1/2 <1 s), sustained by the tetanus toxin (TeTx)-insensitiveexocytosis of small vesicles (diameter <0.1 µm; Kasaiet al., 1999). The latter results, which exclude the involvementof the TeTx target protein, the vSNARE vesicle-associated membraneprotein 2 (Schiavo et al., 1992), differentiate the processfrom the regulated exocytoses of neurosecretory cells, suchas wild-type (wt) PC12 and chromaffin cells, which are TeTxsensitive (Xu et al., 1998; Kasai et al., 1999).

Knowledge about nonsecretory exocytosis is not limited to electrophysiology.Seminal cell biological studies have been carried out by theuse of a monoclonal antibody (mAb) (indicated as antibody) specificfor an exocytic vesicle marker (Borgonovo et al., 2002). Thelatter, identified as a form of the high-molecular-weight proteindesmoyokin/Ahnak (d/A) (Shtivelman and Bishop, 1993; Hashimotoet al., 1995) was shown 1) to be expressed by many, but notall types of cells, of both animal tissues and cultured lines,including those where nonsecretory capacitance responses hadbeen reported: CHO, 3T3, and PC12-27; 2) to be localized atrest within vesicles distinct from other cytoplasmic organelles;and 3) to undergo rapid, TeTx-insensitive transfer to the surfaceof the cell upon stimulation with the Ca²⁺ ionophore ionomycin.Evidence suggested the d/A-positive vesicles to have a rolein the surface enlargements occurring in important processes,such as cell differentiation and plasma membrane repair. Basedon these considerations, the exocytic vesicles marked by d/Awere given the name of enlargeosomes (Borgonovo et al., 2002).

In our previous study (Borgonovo et al., 2002), the electrophysiologicaland cell biological results were assumed to be both due to enlargeosomeexocytosis. However, this identification remained open to question.In fact, the capacitance increases induced by caged Ca²⁺ photolysisseemed to require considerable [Ca²⁺]_i rises (Kasai et al.,1999), much larger than those induced by the ionophore usedin the cell biological studies. Moreover, no comparative resultsexisted about many aspects of the exocytic responses inducedin the same cells by the two types of stimulation. Therefore,the possibility that the responses were due to two parallelprocesses sharing some properties, such as TeTx insensitivity,could not be excluded, also because knowledge about the propertiesof enlargeosomes was still limited.

Here, we report about an integrated electrophysiological/cellbiological investigation of enlargeosome exocytosis and theensuing endocytic process, carried out in the defective PC12-27clone. Our results, on the one hand, document that the Ca²⁺dependence of the responses induced by photolysis and ionomycinis not as different as reported previously, but rather fallsin the same range; on the other hand, they reveal new and unexpectedproperties of the enlargeosome and of its exocytic process anddemonstrate for the first time the postexocytic endocytosisof d/A-positive membranes.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Cloned PC12-27, wild-type (wt) PC12, HeLa cells, and monoclonalantibodies, IgG_2a anti-d/A antibody and IgG_2a anti-chromograninBCIRO, were as in Borgonovo et al. (2002). TeTx and the IgG1anti-lysosomal membrane glycoprotein 1 (Lamp1) monoclonal weregifts from C. Montecucco (University of Padua, Italy) and I.Mellman, (Yale University, New Haven, CT) respectively. TheIgG1 anti-TGN 38 monoclonal and the anti-EEA1 polyclonal werefrom Affinity Bioreagents (Golden, CO); the IgG1 anti-transferrinreceptor monoclonal was from Zymed Laboratories (San FranciscoCA); the IgG1 anti-G58K monoclonal was from Abcam (Cambridge,United Kingdom); the anti-caveolin1 polyclonal and the IgG1anti-flotillin1 monoclonal were from BD Biosciences PharMingen(Heidelberg, Germany); the IgG1 anti-Thy1 monoclonal was fromSerotec (Oxford, United Kingdom); cholera toxin-Alexa fluor488,o-nitrophenyl EGTA (NP-EGTA), and Fura-6F were from MolecularProbes (Eugene,OR);fluoresceinisothiocyanate(FITC)-conjugatedandtetraethylrhodamineisothiocyanate (TRITC)-conjugated goat anti-mouse, goat anti-rabbit,and goat anti-mouse IgG subclasses were from Southern BiotechnologyAssociates (Birmingham, AL); the E2-Link activated peroxidasekit and the Immunopure Fab kit were from Pierce Chemical (Rockford,IL); CypHer5 was from Amersham Biosciences UK, Little Chalfont,Buckinghamshire, United Kingdom; ionomycin was from Calbiochem(Schwalbach, Germany); and other chemicals were from Sigma-Aldrich(St. Louis, MO).

Cell Cultures
Media were supplemented with 2 mM L-glutamine, 100 U ml^–1penicillin, and streptomycin (Cambrex Bio Science Verviers S.p.r.l.,Verviers, Belgium). PC12 wt and PC12-27 were grown in DMEM with10% horse serum (Euroclone, Wetherby, United Kingdom) and 5%fetal clone III serum (Hyclone Laboratories, Logan, UT); HeLacells in the same medium without horse serum and with 10% fetalclone III serum; hybridoma cells in Iscove's modified Dulbeecomedium medium with 10% fetal clone I serum, 5% macrophage conditionedmedium, and 50 µM ${beta}$ -mercaptoethanol.

Patch-Clamp Experiments
Patch pipettes were pulled from borosilicate glass capillaries(GC150F-15; WPI, Sarasota, FL) with a horizontal puller (P-97;Sutter Instrument, Novato, CA) to a resistance of 1–4M ${Omega}$ in a solution containing 100 mM KCl, 10 mM tetraethylammonium-Cl,40 mM KOH/HEPES, 2 mM Na₂ATP, 2 mM MgCl₂, 3.6 mM CaCl₂, 4 mMNP-EGTA, and 0.5 Fura-6F, pH 7.3. In ionomycin experiments,CaCl₂ and NP-EGTA were omitted. The bath contained 130 mM NaCl,5 mM KCl, 1 mM MgCl₂, 30 mM NaOH/HEPES, 4 mM CaCl₂, and 6 mMglucose, pH 7.3. All recordings were made at room temperature.

Membrane capacitance (C_m) and access conductance (G_a), compensatedby C_m and G_a control, were measured by using a SWAM II C (Celica,Ljubljana, Slovenia), operating at 800-Hz lock-in frequencyand by applying a sine voltage of 11-mV rms. The phase anglesetting was determined by applying 1-pF pulses and monitoringtheir projection from the C (signal proportional to Cm) to Goutputs of the lock-in amplifier. C_m, G_a, membrane current,and membrane potential were recorded unfiltered into a PC viaan A/D converter (PCI-6035E; National Instruments, Austin, TX).WinWCP software (John Dempster, Strathclyde University, Glasgow,United Kingdom) was used to acquire and analyze data. Graphswere drawn using the Sigma Plot (SPSS, Chicago, IL).

[Ca²⁺]_i Measurements in Flash Photolyzed and Ionomycin-stimulated Cells
A UV flash from a Xe arc flash lamp (JML-C2; Rapp Opto-Electronic,Hamburg, Germany) was delivered, through an optical fiber toa 40 x fluor oil immersion objective of a Zeiss Axiovert 200microscope, to whole-cell patch-clamped PC12 or PC12-27 loadedwith both NP-EGTA and Fura-6F. The optical pathway includeda combination of two mirrors, the first to merge 85% of flashlight and 15% of fluorescence excitation light (M70-85/15 Rapp;Opto-Electronic, Hamburg, Germany); the second, a dichroic mirror(395 nm), to reflect both lights through the objective to thecell, with the emitted Fura-6F fluorescence passing back tothe photomultiplayer through a 420-nm filter. The Ca²⁺ sensorwas excited by a monocromator at 380 nm, and the emitted lightwas acquired by a Hamamatsu photomultiplier (Till PhotometrySystem, Gräfelfing, Germany); the signal was recorded afterfiltering (300 Hz, 4-pole Bessel). Ionomycin was applied directlyto the extracellular solution. This implied a delay of the effectsof $~$ 30 s that was corrected in the traces. In each cell, [Ca²⁺]_iwas calibrated by measuring autofluorescence (in the cell-attachedconfiguration) and fluorescence (in a resting whole-cell recording)(Kreft et al., 1999).

Differential Centrifugation
Suspensions of PC12-27 in 0.32 M sucrose, 5 mM HEPES, pH 7.4,and protease inhibitors were gently homogenized in a cell cracker(Borgonovo et al., 2002), and the homogenates were centrifugedat 500 rpm for 5 min. The postnuclear pellet and the final supernatantwere obtained by centrifuging the first supernatant at 40,000rpm for 60 min.

Resistance to Nonionic Detergents
The postnuclear pellet, carefully resuspended in 0.32 M sucrose,5 mM HEPES, pH 7.4, and protease inhibitors, was supplementedwith Triton X-100 (TX-100), 0.5% final concentration. After30 min in ice, the preparation was applied to either floatation(Schuck et al., 2003) or top-down (Gagnoux-Palacios et al.,2003) gradients. In the first, loading was in a 1.23 M sucrosecushion (2 ml) at the bottom of a SW 50.1 tube, covered with2 ml of 1.10 M and then with 0.15 M sucrose to volume. In thesecond, the preparation in 0.32 M sucrose was applied in thesame type of tube over two cushions of 1 and 1.3 M sucrose.After 18 h at 46,000 rpm, five fractions and the pellet werecollected from either gradient and processed for Western blotting.

Monolayers of PC12-27 cells in phosphate-buffered saline (PBS),exposed in the cold to 1% TX-100 as described above, were fixedand processed for immunolabeling.

Cholesterol Depletion
Monolayers in the serum-containing medium were treated with3.8 mM methyl- ${beta}$ -cyclodextrin (cdx) for 10–50 min, and then0.5 µg/ml cholera toxin-Alexa fluor488 was added (to monitorits endocytosis; Wolf et al., 2002) and the incubation was pursuedfor 10 min. After 5-min treatment with 3 µM ionomycinor its solvent, cells were fixed and immunolabeled. For SDS-PAGE,cell processing was similar, but cholera toxin and ionomycinwere not added.

SDS-PAGE and Western Blotting
Resuspended monolayers were solubilized in ice-cold medium containing50 mM HEPES, pH 7.5, 150 mM NaCl, 15 mM MgCl₂, 1 mM EGTA, 10%mM glycerol, and 1% TX-100, and then quickly centrifuged at20,000 x g for 5 min to eliminate nuclei. Protein was assayedwith bicinchoninic acid. For detergent resistance experiments,fixed volumes of the gradient fractions were loaded for SDS-PAGE;otherwise, fixed amounts of protein were loaded. For Westernblotting, gels transferred to nitrocellulose filters were firstblocked for 1 h with 5% nonfat dry milk in Tris-buffered saline(TBS), and then incubated for 3 h with the primary antibodydiluted in PBS with 3% bovine serum albumin (BSA), washed inTBS (5-fold for 10 min), incubated for 1 h with the peroxidase-conjugatedsecondary antibody (1 µg ml^–1), washed again inTBS as described above and once in PBS, and developed by chemiluminescence(ECL Western blotting detection; Amersham Biosciences UK). Signalswere acquired by Personal Densitometer SI and Image Quant (AmershamBiosciences).

Immunofluorescence and Imunoelectron Microscopy
For cell surface immunofluorescence, monolayers plated on poly-(L-lysine)–coatedcoverslips, at rest or after ionomycin treatment (0.1–5µM; 0.5–5 min), treated with or without drugs and/orcholera toxin as indicated in figure legends, were fixed onice for 10 min with 4% paraformaldehyde in PBS, pH 7.4, quenchedwith 0.1 M glycine, and then washed in PBS containing 0.3% BSAand 20% goat serum. The latter solution also was used for furtherwashes and to dissolve antibodies. Exposure to the primary antibodieswas for 2 h at 22°C, and then monolayers were washed extensively,exposed for 2 h to FITC- or TRITC-conjugated secondary antibodies,washed, mounted and analyzed. For quantitations, monolayerswere processed as described above except that nuclei were labeledwith 4,6-diamidino-2-phenylindole (DAPI). For establishing thecell percentage that had undergone exocytosis in 5-min applicationof various concentrations of ionomycin, d/A-positive and -negativecells were counted under blind conditions; for measuring quantitativelythe d/A surface labeling at rest and after stimulation, theintensity of the signal in individual surface-labeled cellswas established making reference to an arbitrary scale of sixvalues, and the average score ± SE of 30–40 cellgroups was calculated and expressed as percentage of the topfluorescence value. For the time course of the ionomycin-inducedexocytic responses, parallel monolayers were fixed by rapidaddition of paraformaldehyde (4% final concentration) at differenttimes after application of 3 µM ionomycin and processedas described above. The labeling intensity of cell groups wasestablished as described above.

For whole-cell immunofluorescence, the monolayers, fixed andquenched as described above, were washed with the PBS-BSA-goatserum solution with 0.3% TX-100. Treatment with antibodies wasas for surface immunolabeling, except that the solution andwashing PBS always contained 0.3% TX-100. In some experiments,the cells were processed by a combination of surface and whole-cellimmunolabeling, i.e., they were first surface immunolabeledwith antibody, and then permeabilized and whole-cell immunolabeledwith other primary antibodies.

Immunofluorescence experiments of endocytosis were carried outas for surface immunolabeling, except that 1–5 µMionomycin was administered at 37°C in the presence of antibodyfor 5–30 min. Monolayers were then washed, fixed, quenched,permeabilized, and labeled by the secondary antibody. In somesurface and endocytosis experiments, the cells, after d/A immunolabelingand fixation, were washed with the PBS-BSA-goat serum supplementedwith 0.3% TX-100 and then dually labeled for another markerfollowing the whole-cell immunofluorescence protocol. Dual immunolabeledsamples were analyzed quantitatively for colocalization of d/Awith specific markers by using the ImageJ software to establishthe fraction of pixels dually labeled above a threshold, accordingto the formula (dually labeled)*(d/A-labeled)^–-1*100.

Immunofluorescent cells were studied using Bio-Rad MRC 1024and Leica SP2 AOBS confocal microscopes. For image deconvolutionaimed at blur removal and tridimentional cell reconstruction,optical sections, taken every 150 nm with a wide field microscopeon the Delta Vision system, were analyzed with the soft WoRxDeconvolve software (Applied Precision, Washington, DC).

Electron microscopy of immunoperoxidase endocytosis was carriedout as for immunofluorescence, except that antibody was conjugatedto horseradish peroxidase whereas fixation was with 2% glutaraldehyde-4%paraformaldehyde. The diaminobenzidine reaction was carriedout according to Ochs and Press (1992), except that H₂O₂ (0.03%)was included in the mixture, and the reaction was arrested after20 min by washing with Tris buffer. Reacted monolayers werewashed with cacodylated buffer, postfixed in 1% OsO₄ for 10min, dehydrated, embedded in Epon, and examined in a HitachiH7000 electron microscope.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

The clone of the rat pheochromocytoma PC12 cell line used here,PC12-27, is advantageous for the present studies: it is richwith enlargeosomes (Borgonovo et al., 2002); it maintains mostof the molecular and structural properties typical of wt PC12,a neurosecretory line devoid of enlargeosomes, which can thereforebe used for reference; it is specifically defective of the neurosecretionprogram, in particular it fails to express both types of neurosecretoryorganelles, synaptic-like microvesicles (SLMVs) and dense granules(DGs), as well as the plasmalemma and soluble proteins instrumentalto their exocytic discharge (Malosio et al., 1999; Grundschoberet al., 2002); and it is very poor of lysosome exocytosis (Borgonovoet al., 2002). Therefore, the participation of lysosomes tothe cell surface enlargement induced by stimulation is negligible.

Ca²⁺ Dependence and Kinetics of the Nonsecretory Exocytosis
Our first aim was to establish whether in PC12-27 the rapidsurface increase induced by photolysis of a caged Ca²⁺ compound,revealed by patch-clamp capacitance assay, occurs only in responseto the high [Ca²⁺]_i rises (50 µM or above) previouslyused by Kasai et al. (1999). These rises are much higher thanthose (a few micromolar only) induced by the Ca²⁺ ionophoreionomycin, which nevertheless are sufficient to trigger enlargeosomeexocytosis, as revealed by the surface appearance of d/A, theenlargeosome marker (Borgonovo et al., 2002).

To answer this question we replaced the previously used cagedCa²⁺ compound dimethoxynitrophenamine tetrasodium salt (DM-nitrophen)with another compound of lower Ca²⁺ affinity, NP-EGTA, whoseinduced [Ca²⁺]_i changes can be kept low, similar to those attainedwith ionomycin (Yang et al., 2002). The capacitance responsesinduced by photolysis of NP-EGTA (maximal increases $~$ 8% abovethe resting surface area; Figure 1c) were investigated in boththe neurosecretory wt PC12 and in the defective PC12-27. Theresponses of the first were biphasic, composed by an initialsmall peak, possibly due to the exocytosis of SLMV, followedby the slower, higher, and more persistent increase due to DGs(Figure 1a). Both these increases were almost completely blockedby the intracellular perfusion of TeTx (Figure 1c). In contrast,in the defective PC12-27 the increases of capacitance were rapid,monophasic (Figure 1b), and unaffected by TeTx (our unpublisheddata). PC12-27 cells stimulated by photolysis of NP-EGTA alsowere processed for surface immunofluorescence to reveal enlargeosomeexocytosis. As can be seen in Figure 1d, a cell fixed with paraformaldehydea few seconds after photolysis seemed already surface positivefor the specific marker d/A, documenting that enlargeosome exocytosishad quickly taken place.

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Figure 1. NP-EGTA photolysis-induced exocytosis in wt PC12 and PC12-27 cells. (a and b) [Ca²⁺]_i increases and the ensuing plasma membrane capacitance responses induced by photolysis of the caged Ca²⁺ compound in representative wt PC12 and PC12-27 cells, respectively. The biphasic capacitance trace of the wt PC12 (a) is probably accounted for by the rapid exocytosis of SLMVs followed by the slow exocytosis of DGs; the rapid response of the PC12-27 cell (b) may be sustained, entirely or in part, by the exocytosis of enlargeosomes. In agreement with this possibility, PC12-27 cells fixed a few seconds after photolysis and then immunolabeled, show an intense surface positivity for d/A (d). (c) On average, the maximal capacitance increase (expressed as percentage of the cell surface area at rest) was approximately the same in wt and defective PC12 cells and in wt PC12, this response was blocked by tetanus toxin (4 µM inside the pipette; Xu et al., 1998

). The bars in d and in all immunofluorescence panels of the subsequent Figures correspond to 10 µm.

Figure 2 shows results obtained in PC12-27 cells treated with3 µM ionomycin. With this drug, the [Ca²⁺]_i rises wereslow and were followed by delayed increases of capacitance,irregular in their outline (possibly due to the coexistenceof some endocytosis), reaching plateaus within 3–4 min(Figure 2a; see also Huang and Neher, 1996). These traces werecompared with the quantized surface immunolabeling responsesinduced by the ionophore, administered for different times (30s to 5 min), followed immediately by quick fixation and immunodecorationof the cells. As can be seen in Figure 2b, the increase of thesurface d/A signal induced by ionomycin followed a kineticssimilar to that of the capacitance responses. As far as theconcentration dependence, d/A became appreciable at the surfaceof a few PC12-27 cells already at 0.1 µM ionomycin (average[Ca²⁺]_i $~$ 1.0 µM). At 3 µM and above, the majorityof the cells seemed positive (Figure 2c), most often showingstrong immunolabeling signals (Figure 2d; Borgonovo et al.,2002).

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Figure 2. Ionomycin-induced exocytosis in PC12-27 cells. (a) Increase of capacitance that follows the [Ca²⁺]_i rise in a representative cell exposed to ionomycin (3 µM, arrow). Notice the slow rate of both responses and the irregular outline of the capacitance trace, which could be due to concomitant membrane endocytosis. The capacitance bar of 500 fF corresponds to $~$ 2.5% of the initial cell surface area. (b) Time course of the d/A surface appearance, given for each time point as the average fluorescence intensity in a population of 30–40 cells exposed to ionomycin for the indicated times, and then rapidly fixed and surface immunolabeled without permeabilization. Notice that the curve of this panel, expressed in percentage of the top value of the scale, resembles roughly the capacitance trace of a. The last point of the trace corresponds to 300 s of stimulation. (c) Concentration dependence of the ionomycin-induced d/A surface appearance, expressed as the percentage of positive cells in a population of scanned PC12-27. In the positive cells, the intensity of the surface fluorescence signal did not remain the same but increased considerably as a function of the ionomycin concentration, in parallel to the percentage of cell positivity, reaching high values such as those of d, which shows cells exposed to 3 µM ionomycin for 5 min.

The Enlargeosome Membrane Is Resistant to Nonionic Detergents
So far, little was known about the enlargeosome membranes. Inparticular, their resistance to nonionic detergents, a propertydependent on the cholesterol and phospholipid composition, hadnot been investigated. A postnuclear particulate fraction wastherefore resuspended in 0.5% TX-100 at 4°C and analyzed30 min later by both floatation (Figure 3) and top-down (ourunpublished data) sucrose gradient centrifugation, with consistentresults. As can be seen in Figure 3, c and d, the markers oforganelles known to be mostly solubilized by TX-100, i.e., transferrinreceptor (recycling endosomes; Figure 3d) and G58K (Golgi cisternae;Figure 3c), were recovered almost completely in the dissolved,nonfloated fractions 4 and 5, whereas the endoplasmic reticulum(ER) chaperone proteins calreticulin and calnexin (Figure 3d),and especially the trans-Golgi network (TGN) marker TGN38 (Figure 3c),exhibited a dual distribution, with similar recovery inthe dissolved and in the floated 2 and 3 fractions (shadowedareas in Figure 3). In contrast, well known markers of resistantmembranes, caveolin1 (van Deurs et al., 2003) and Thy1 (alsoknown as CD90) (Simons and Toomre, 2000), were recovered mostly(>65%) in the floated fractions (Figure 3b) together withonly 20% of total protein (Figure 3a). In the case of flotillin1,another recognized resistance marker (Bickel et al., 1997),the recovery in the dissolved fractions 4 and 5 ( $~$ 30%) was higherand that in the resistant fractions 2 and 3 (<50%) lowerthan those of caveolin1 and Thy1 (Figure 3b). The recovery ofd/A, on the other hand, was similar to that of the latter tworesistance markers (Figure 3a). Consistently, the d/A immunofluorescencepattern was apparently unchanged by the TX-100 treatment appliedto PC12-27 cells before fixation (compare in Figure 3, f and e),whereas in the same cells the transferrin receptor immunofluorescencewas completely removed by the treatment (our unpublished data).

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Figure 3. Effects of TX-100 on the distribution of d/A in a floatation gradient, compared with other membrane markers, and on the d/A immunolabeling of PC12-27 cells. The fractions of the floatation gradient (a–d) were analyzed by Western blotting. Of the fractions, P is the pellet, 5 and 4 include the components solubilized by TX-100, 3 and 2 (shadowed) are the detergent-resistant fractions, and 1 is the top, 0.15 M sucrose layer. The SDS-PAGE slots of all lanes except 1 were loaded with 100-µl samples of the fractions recovered from the gradient. Values are given as percentage of recovery of the markers in the various fractions. The traces in a refer to d/A and total protein (tp); those in b to caveolin (Cav), Thy1 and flotillin1 (Flot); those in c to the Golgi (G58K) and TGN (TGN38) markers; those in d to the transferrin receptor (TFR), and the endoplasmic reticulum proteins calnexin (Cnx) and calreticulin (CR). (e and f) d/A immunolabeling of PC12-27 cells fixed before (e) and after (f) treatment with TX-100 (1%, 30 min at 4°C) and then processed for whole-cell immunofluorescence.

The detergent resistance of d/A opened the possibility of enlargeosomesto be one of the known organelles specific for the resistancemarkers. Previous studies with anti-TGN38 and anti-ER markershad already excluded the colocalization of antibody with thecorresponding antigens (Borgonovo et al., 2002). As far as theother markers (Figure 4, a–c; quantitative data in Figure 4d),an apparent minor d/A colabeling was observed in PC12-27with both Thy1 (Figure 4b) and flotillin1 (Figure 4c), whereaswith caveolin1 (investigated in HeLa cells, which are also richof enlargeosomes; Borgonovo et al., 2002), because the availableantibody recognized poorly the fixed rat protein of PC12-27,the immunolabeling pattern seemed almost completely distinctfrom that of the enlargeosome marker, which was similar to thatof PC12-27 (Figure 4a).

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Figure 4. Dual immunolabeling of HeLa and PC12-27 cells for d/A (red) and raft markers (green). (a–c) HeLa (a) and PC12-27 (b and c), investigated by whole-cell immunolabeling while at rest. d/A puncta, localized primarily in the superficial layers of the cytoplasm, show very little apparent colocalization with caveolin1 (a), localized primarily at the cell surface. With Thy1 (b), and, especially, with flotillin1 (c), which are distributed to the whole cytoplasm, the apparent colocalization is still low but more pronounced than with cavolin1. The flotillin1 immunolabeling of the nucleus is an artifact. In d, the apparent colocalization of the three raft markers with d/A in the cytoplasm of groups of 10 resting cells is given in quantitative terms. The HeLa cells (e) and the PC12-27 cells (f and g) were stimulated with ionomycin (3 µM, 5 min). After fixation they were first surface immunolabeled for d/A, and then permeabilized and whole-cell labeled for the other markers. Under these conditions, therefore, apparent colocalization can be observed only at the cell surface. Notice that such a colocalization of d/A with caveolin1 (e) is very low, with Thy1 (f) is larger but variable, whereas with flotillin1 (g) it is considerable, as confirmed by the quantitative analyses of h, which refers only to the cell surface. For the Thy1-d/A surface colocalization, also see Supplemental Material Video I, showing a tridimensional rendering.

Immunolabeling of membrane-resistant markers was carried outalso in ionomycin-stimulated cells. To focus on the surface-exposedd/A and compare its distribution with that of the other markers,which are not exposed to the extracellular space, we used thecombined protocol of surface and whole-cell immunolabeling,i.e., fixed cells were first exposed to antibody, then permeabilizedand finally exposed to the primary antibody against one of thethree investigated markers. As can be seen in the images ofFigure 4, e–g, and in the corresponding quantitative dataof Figure 4h, no coincidence was observed between exocytizedd/A and caveolin1 (Figure 4, e and h). In contrast, some ofthe stimulation-induced d/A surface labeling seemed to coincidewith Thy1 (Figure 4, f and h) and especially with flotillin1(Figure 4, g and h). Part of this coincidence remained evidentafter deconvolution of the images (see Supplemental MaterialVideo I for a tridimensional rendering of the surface interactionbetween Thy1 and d/A).

Cholesterol Depletion Does Not Inhibit Enlargeosome Exocytosis
In view of their detergent resistance, enlargeosome membranesseem to be rich in cholesterol. We therefore investigated whether,and to what extent, the structure and function of the vesicleare affected by incubation of PC12-27 cells with the cholesterol-extractingagent cdx (3.8 mM) for up to 60 min. During the last 10 minof the cdx treatment, cholera toxin-Alexa fluor488 was addedto monitor an independent process, toxin endocytosis (Wolf etal., 2002). In PC12-27 cells, the latter process is inhibitedalmost completely by 1-h incubation with cdx (compare Figure 5, a and c;see also Supplemental Material Figure 1), in parallelwith the drop of cholesterol revealed by cell labeling withfilipin (our unpublished data). In contrast, endocytosis ofthe transferrin receptor is unaffected by cdx (our unpublisheddata).

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Figure 5. Effects of cholesterol depletion on enlargeosome exocytosis. PC12-27 cells, pretreated (c and d) or not (a and b) with cdx for 60 min, were all exposed to cholera toxin-Alexa488 (green) during the last 10 min of the pretreatment, followed (b and d) or not (a and c) by ionomycin stimulation (3 µM, 5 min). After fixation the cells were surface immunolabeled for d/A (red). Notice that in the cells not treated with cdx (a and b), the endocytosis of cholera toxin (green) was intense. The surface d/A labeling was inappreciable in the cells in a, as in all resting PC12-27 cells (Borgonovo et al., 2002

), and became clearly evident after ionomycin (red and yellow labeling of b). After cholesterol depletion (c and d), the general PC12-27 phenotype was altered, with flattening and or/shrinkage of the cell body. Endocytosis of cholera toxin was blocked (lack of green labeling). A clear surface d/A signal (red) was visible already in the resting cells (c) and was increased by ionomycin to levels similar to those of stimulated controls (compare d with b). (e) Quantitative summary (as in Figure 2b) of the surface d/A-labeling results obtained in groups of 10 cells from the populations illustrated in a–d.

Cholesterol-depleted PC12-27 cells exhibited some structuralalterations, such as flattening and/or shrinkage of the cellbody with redistribution of the enlargeosomes from the subplasmamembrane area to the whole cytoplasm, accompanied by their partialaggregation in one or a few large clumps (Supplemental MaterialFigure 1, compare e and f to d; and Video II for a deconvolutionanalysis). Within living cells, however, most enlargeosomeswere not disrupted, as documented by the good preservation ofthe d/A band in Western blots prepared from total cell preparations(Supplemental Material Figure 1g; Borgonovo et al., 2002). Incontrast, in Western blots prepared from gently homogenized,cdx-pretreated cells (but not from control cells), the d/A bandseemed converted into a ladder (Supplemental Material Figure1h). This suggests that the cholesterol-depleted organelleshad not resisted the homogenization insult, releasing the markerthat was then cleaved by cytosolic proteases.

Exocytosis of enlargeosomes was not blocked by cholesterol depletion.Compared with control cells, where cholera toxin endocytosiswas considerable (Figure 5, a and b) and only little surfaced/A labeling was visible before stimulation (Figure 5, a and e),the cdx-treated cells showed a progressive decrease of choleratoxin endocytosis (Figure 5, c and d; Supplemental MaterialFigure 1, a–c) accompanied by an increase of the restingd/A surface signal (Figure 5, c and e). The latter, however,was still reinforced by ionomycin (3–5 µM), appliedfor 5 min after 60 min of cdx treatment, to an extent similarto that of cdx-untreated cells (compare Figure 5, b and d; Figure 5e).We conclude that cholesterol depletion affects the trafficof enlargeosome membranes at the surface of resting cells withoutinhibiting significantly the responses induced by the Ca²⁺ ionophore.

Postexocytic Endocytosis
In the previous patch-clamp studies, the capacitance increasestriggered in PC12-27 cells by photolysis of DM-nitrophen persistedin all cases until the end of the recordings (Kasai et al.,1999). Whether this was due to a lack of endocytosis or whetherit was an artifactual consequence of the high [Ca²⁺]_i risesinduced in the cells to stimulate exocytosis remained unclear.To investigate this point, a systematic analysis was carriedout in PC12-27 cells stimulated at lower [Ca²⁺]_i by photolysisof NP-EGTA. Figure 6a illustrates a photolyzed cell ([Ca²⁺]_i $~$ 4 µM), representative of an $~$ 60% subpopulation of analyzedcells, in which the increased capacitance remained almost stableduring the first 30 s after photolysis and was largely unaffectedby the application of further photolysis flashes inducing additional[Ca²⁺]_i increases. On the contrary, the cells in Figure 6, b and c,representative of the remaining subpopulation, showedappreciable declines of the NP-EGTA photolysis-induced capacitanceincreases, which were accelerated by further photolysis flashes(Figure 6c). These observations suggested that, at least inthe second subpopulation, postexocytic endocytosis is regulatedby [Ca²⁺]_i in the 3–5 µM range. Indeed, in the cellswhere photolysis had induced relatively low [Ca²⁺]_i rises (average3.76 ± 0.25 µM; n = 5) the subsequent capacitancedecreases were slow ( $~$ 30 fF/s) and only partial during the firstminute (Figure 6, d and e), whereas in those with higher [Ca²⁺]_irises (average of 4.82 ± 0.24 µM; n = 5), the rateof decline was almost fourfold faster, and the values reachedat 0.5–1 min after stimulation were close to resting (Figure 6, b–e).

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Figure 6. Time course of capacitance after the stimulation-induced rise in PC12-27 cells: Ca²⁺ dependence of endocytosis. The three representative cells in a–c show jumps of [Ca²⁺]_i to $~$ 4 µM induced by NP-EGTA photolysis causing parallel capacitance rises of $~$ 600-2000 fF. In the cell of a, the increased capacitance remains largely stable, insensitive to further photolysis-induced [Ca²⁺]_i spikes. This cell belongs to the subpopulation in which endocytosis is delayed. In contrast, b and c show cells of the subpopulation in which endocytosis begins during the first minute. Notice that the rate of the process is faster in c, where subsequent photolysis spikes prevent the decrease of the [Ca²⁺]_i. The data in d and e illustrate the Ca²⁺ dependence of the endocytic process. Compared with a group of five cells reaching maximal [Ca²⁺]_i levels <4 µM (average 3.76 ± 0.25 µM), five cells reaching levels >4.5 µM (average 4.82 ± 0.24 µM) exhibit endocytic rates more than fourfold faster (d). Therefore, 30 s after stimulation, the average capacitance values of these cells correspond to an 82% decrease from the exocytic peak (e), i.e., they have returned near the resting values, whereas the average values of the lower [Ca²⁺]_i group have decreased of only 38%. (f) Time course of the capacitance in a representative cell stimulated with ionomycin (3 µM) administered at the arrow. Notice the irregularities of the trace which declines slowly and remains away from the resting values for the whole recording time (several minutes).

In the cells stimulated with ionomycin, on the other hand, alarge poststimulatory capacitance decline was never observedas long as the recording could be pursued (several minutes).Rather, the rate was slow and the decline was only partial.Irregularities of the traces, already mentioned during the initialcapacitance rise, persisted and increased in the cells duringdecline (Figure 6f). Together with the data of Figure 2a, theseresults may suggest that, in the course of the ionomycin treatment,exo- and endocytosis take place concomitantly, with predominanceof exocytosis during the first few minutes and of endocytosisthereafter.

d/A Endocytosis by Nonacidic Endosomes
The capacitance results of Figure 6 document that, in a significantfraction of stimulated PC12-27 cells, poststimulatory endocytosistakes place within the first minute. However, they provide noinformation about the nature and properties of the endocyticvesicles. To investigate whether the membrane exhibiting theenlargeosome marker d/A participates in the endocytosis, livingcell monolayers were first exposed to antibody, its monovalentfragment (Fabantibody), or an unspecific antibody applied withor without ionomycin (3 µM) for 0.5, 5, and 30 min at37°C, and then cooled at 4°C, washed extensively, andfinally fixed. The intracellular distribution of the endocitizedantibodies was revealed by staining with the secondary antibodyapplied after membrane permeabilization with TX-100 and stainingof nuclei with DAPI. No intracellular immunolabeling was appreciablein nonstimulated cells incubated for up to 30 min with eitherthe antibody or the control, anti-chromograninB antibody (ourunpublished data). Likewise, no labeling was observed when thelatter antibody was applied as described above, however togetherwith ionomycin (Figure 7d). In contrast, with antibody and Fab-antibody,similar patterns were observed, composed of puncta, initiallysmall and distributed close to the surface of a few cells, latermore and more numerous, enlarged and much more frequent in thecell population (Figures 7, b and c, and Figure 8). We concludethat, in PC12-27 cells, the enlargeosome marker d/A is involvedin the poststimulatory endocytosis.

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Figure 7. d/A endocytosis in ionomycin-stimulated PC12-27 cells. The panels show the cellular distribution of antibody applied to living cells together with ionomycin for 0.5 (a), 5 (b), and 30 (c) min. Notice that at the early time point, only a small fraction of cells shows intracellular accumulation of d/A-positive puncta. Later, the number of positive cells increases and the number and intensity of their puncta also increase, reaching considerable apparent size at 30 min. With a control mAb, against a protein not expressed by PC12-27 cells (chromograninB), incubated with ionomycin (d) or without (our unpublished data), no intracellular labeling was observed.

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Figure 8. Endocytic organelles positive for d/A are distinct from the TGN, classical endosomes, and lysosomes. The panels show groups of PC12-27 cells exposed to ionomycin (3 µM) together with antibody (red) for 30 min, and then fixed and whole-cell labeled (green) for the TGN marker TGN38 (a), the sorting endosome marker EEA1 (b), the recycling endosome marker transferrin receptor (c), and the lysosome marker Lamp1 (d). Merging of the images of the dually labeled cells reveals only very low levels of apparent coincidence, documenting a lack of colocalization of d/A with the investigated markers. Notice also that the overall distribution of the d/A-positive endosomes in the cytoplasm is mostly peripheral not only with respect to the TGN and recycling endosomes but also to sorting endosomes and lysosomes. The green staining of nuclei in b is an artifact of the polyclonal anti-EEA1 antibody used.

Differential properties of the d/A-positive endosomes were investigatedby dual immunofluorescence with respect to specific markers:the early endosome antigen 1 (EEA1; Figure 8b) and the transferrinreceptor (Figure 8c), known to reside in the two classes ofthe coated vesicle-derived endosomes, the sorting and the recyclingendosomes, respectively (Maxfield and McGraw, 2004); TGN38 (Figure 8a)and Lamp1 (Figure 8d), the markers of TGN and lysosomes,where endosomes and endosomal proteins are often addressed.In all analyzed cells the d/A-positive puncta (red) were preferentiallydistributed to the cytoplasmic layers in the proximity of thecell surface, with no obvious overlapping with the other markers(green in Figure 8, a–d). The latter, on the other hand,exhibited their well known distribution: clustering in juxtanuclearareas for TGN38 (Figure 8a) and the transferrin receptor (Figure 8c);the superficial cytoplasmic layers for EEA1 (Figure 8b);a wide scattering throughout the cytoplasm for Lamp1 (Figure 8d).The lack of colocalization of these markers with d/A punctawas confirmed by a quantitative analysis of groups of 10 cellsselected at random. In these groups, in fact, apparent coincidencedid not exceed average values (<10%) attributable to thelow resolution power of confocal microscopy.

Subsequent experiments were carried out to establish whetherthe lumen of the d/A-positive endosomes is acidic, as it isthe case of classical endosomes and lysosomes, or whether, incontrast, it is neutral. To investigate the problem, antibodywas coupled to a pH-sensitive dye, CypHer5, which is unstainedin the neutral and turns red in the acidic environment (Adieet al., 2003). Parallel experiments were carried out for referencewith the dye coupled to the antibody against the lysosomal markerLamp1. Figure 9a shows PC12-27 cells stimulated for 30 min withionomycin in the presence of antibody-CypHer5, subsequentlyfixed, permeabilized, and stained with the FITC-conjugated secondaryantibody. As can be seen, these cells exhibited numerous punctathat were all green. The results indicate that, in the endocyticorganelles reached by d/A during the 30-min incubation, CypHer5remains unstained, i.e., that the organelle lumen is neutral.In contrast, when the 30-min ionomycin stimulation was carriedout in the presence, not of antibody but of Lamp1-CypHer5, thecolor of puncta was yellow (Figure 9b), as expected by the combinationof the green of the FITC-secondary antibody with the red acquiredby CypHer5 in the acidic environment of lysosomes. Similar results—greenpuncta with antibody-CypHer5 and yellow puncta with anti-Lamp-CypHer5—wereobtained in further, longer incubation experiments carried outwith and without stimulation by ionomycin. The results obtainedin unstimulated PC12-27 cells incubated for 24 h with eitherantibody-CypHer5 or anti-Lamp1-CypHer5 are shown in Figure 9, c and d,respectively. The neutral lumen, therefore, is notonly a property of the d/A-positive, postexocytic endosomesbut also of the organelles where the enlargeosome marker isrecovered long time after endocytosis. Together with the duallabeling data of Figure 8, these results confirm that the d/A-richendocytic/recycling organelles are distinct from classical endosomes/lysosomes.

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Figure 9. Distribution of either CypHer-antibody or CypHer-anti-Lamp1 applied to PC12-27 cells during stimulation with ionomycin for 30 min (a and b) or while resting for 24 h (c and d). Notice that the organelles where antibody and anti-Lamp1 antibody accumulate exhibit different color labeling because of their different lumenal pH. The d/A-positive puncta (a and c) are all green, due to the antibody immunolabeling only. In these puncta, therefore, CypHer is unstained, i.e., the lumen of the organelle is neutral. In contrast, the Lamp1-positive organelles, the lysosomes, are yellow (b and d), resulting from the merge of the green of the Lamp1 immunolabeling with the red that CypHer acquires in the acidic environment of the lumen.

The investigation of d/A endocytosis was pursued at the ultrastructurallevel. Previous attempts of enlargeosome immunoelectron microscopyhad been largely unsuccessful because, after fixation with evenlow concentrations of glutaraldehyde, the antigen is poorlyrecognized by antibody (Borgonovo et al., 2002). In the presentstudy, we focused on the distribution and morphology of theorganelles labeled by peroxidase-coupled antibody applied for5–30 min to living PC12-27 cells during ionomycin stimulation.With the control mAb (against chromograninB, which is not expressedby PC12-27), administered at the same concentration and forthe same times of antibody, no detectable intracellular labelingwas observed (our unpublished data). In contrast, with antibodycytoplasmic organelles were labeled, although to variable extent.In the intensely positive cells, weakly labeled vesicles wereaccompanied by more numerous, distinctly larger (diameters between80 and 150 nm), and strongly labeled profiles, often of irregularshape (Figure 10, a and c), that could be clustered in groupsin the proximity to plasma membrane (Figure 10b). Deeper inthe cytoplasm, the organelle labeling was intense, concentratedprimarily into vacuoles (300–600 nm in diameter), someof which containing discrete vesicles (Figure 10, c–f).These vacuoles often showed small, coated bulges, looking asbudding vesicles (Figure 10, d and e). In the Golgi/TGN area,d/A-positive organelles were absent.

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Figure 10. Ultrastructure of d/A-positive endocytic organelles decorated by antibody-peroxidase. PC12-27 cells were incubated with antibody-peroxidase together with ionomycin as in Figure 7. Various forms of the d/A-positive organelles are shown in the panels. In a, three positive organelles, 100–300 nm in diameter, are distributed individually in the subplasmalemma area, at 1–1.5 µm distance from each other; in b, small (80–100 nm), lightly labeled profiles are clustered in the proximity of the plasma membrane together with larger, more intensely labeled vesicles; c shows at the top a small positive vesicle, with an organelle of 150 nm diameter and a larger irregular vacuole containing a few segregated vesicles located in the proximity, but not inside the Golgi/TGN area. Even larger, irregular vacuoles containing vesicles and with coated bulges, likely corresponding to budding vesicles (asterisks), are shown in d and e. The latter panel includes also another positive organelle and a vesicle. Finally, f shows an enlargement of the vacuole of e, illustrating the distribution of the DAB precipitate apposed to the lumenal face of the limiting membrane. Examples of the periodic pattern of peroxidase labeling of the vesicle and vacuole lumenal membrane surface are visible in all panels. In contrast to the d/A-positive organelles, the coated pits and vesicles (arrows and arrowheads in c and e) are all d/A negative. Bars, 0.5 µm, except in d and f, where bars are 0.2 µm. GC, Golgi complex.

In the labeling conditions used, the diamino benzidine precipitatewas always distributed in direct contact with the inner faceof the organelle limiting membrane. Interestingly, the decorationseemed not random but distributed according to a pattern composedby rows of puncta aligned at $~$ 40 nm, center-to-center distancefrom each other (Figure 10, a–e). This decoration patternmight be related to the structure of the d/A protein, composedby two terminal domains connected by >30 internal repeats(Shtivelman and Bishop, 1992), each including a site for antibodybinding (Borgonovo et al., 2002).

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

The occurrence in various cell types of regulated, nonsecretoryexocytoses, taking place in response to large [Ca²⁺]_i increasesand inducing considerable surface enlargements, had been shownseveral years ago by patch-clamp capacitance studies (Coorssenet al., 1996; Ninomiya et al., 1996; Kasai et al., 1999). Morerecently, the search for the corresponding vesicles lead tothe discovery of enlargeosomes, identified by their lumenalmarker, the high-molecular weight, peripheral membrane proteind/A (Shtivelman et al., 1992; Shtivelman and Bishop, 1993; Hashimotoet al., 1995), which upon exocytosis remains bound to the cellsurface (Borgonovo et al., 2002). So far, however, the exocytosesrevealed by capacitance and those revealed by immunocytochemistrywere investigated separately. On the one hand, some of theirproperties seemed common: both are due to small vesicles andboth are Ca²⁺ dependent and insensitive to TeTx; on the otherhand, one had been triggered rapidly (t_1/2 < 1 s) by high[Ca²⁺]_i jumps (50 µM and above; Kasai et al., 1999), theother was much slower and occurred already at low micromolar[Ca²⁺]_i (Borgonovo et al., 2002). Although very suggestive,therefore, the possibility that they are due to the same processwas still open to question.

The results we have obtained by a combined, capacitance/immunocytochemicalinvestigation strengthen the single process hypothesis, solvingin particular the problem of the different Ca²⁺ dependence.By replacing the high-affinity caged Ca²⁺ compound DM-nitrophenwith the lower affinity NP-EGTA, we showed that [Ca²⁺]_i risesmuch lower than those reported previously are sufficient totrigger the capacitance responses, i.e., they fall in the samerange of those induced by ionomycin, the Ca²⁺ ionophore mostlyused in the immunocytochemical studies. Moreover, the d/A exocyticresponses induced by the ionophore were shown to develop concomitantlyto slow, but considerable capacitance rises, following the [Ca²⁺]_iresponses. It should be mentioned, however, that because theincrease of the cell surface area induced by exocytosis of thed/A-positive vesicles could not be evaluated quantitatively,we cannot exclude that only part of the capacitance responsesare accounted for by enlargeosomes, the rest being due to other,so far unknown exocytic organelles, exocytized in parallel andwith similar properties.

Our results extend significantly our knowledge about enlargeosomesand their cellular role. The low micromolar [Ca²⁺]_i dependenceof their exocytosis expands the range of physiological and pathologicalprocesses in which these vesicles could be involved. Some ofthese processes, cell differentiation and membrane repair, havealready been identified (Borgonovo et al., 2002; Cerny et al.,2004). Moreover, the enlargeosome membranes were found to beresistant to nonionic detergents, a property attributed to theexistence, in the plane of their membrane, of small microdomains(<100 nm in diameter), the rafts, rich in cholesterol andsphingolipids (Pralle et al., 2000; Simons and Toomre, 2000;Anderson and Jacobson, 2002; Parton and Hancock, 2004), wherespecific proteins accumulate in a dynamic equilibrium with theother membrane domains (Kenworthy et al., 2004). Extensive evidencein various organelles and processes (especially the TGN; endocytosis;constitutive exocytosis) has demonstrated the key role of raftsin membrane dynamics (fusions, fissions, trafficking, and interactions:for reviews, see Nichols, 2003; Helms and Zurzolo, 2004; Mayorand Rao, 2004). The abundance of rafts, as observed in enlargeosomes,is not common among the organelles competent for regulated exocytosisand could therefore play specific roles at various steps ofthe new vesicle life, including (in addition to exocytosis,which is discussed below): generation, presumably at specificdomain(s) of the TGN (Gkantiragas et al., 2001; Maxfield, 2002;Gleeson et al., 2004); traffic and possible interactions, homologousand possibly also heterologous with other membrane systems.The recognition of the extensive detergent resistance, the firstgeneral property of the enlargeosome membrane so far identified,could serve in the study of these processes, for example, byproviding criteria for the isolation and characterization ofthe vesicles together with important cues and tools for theinterpretation of future results.

As a direct fall-out of membrane resistance results, we exposedthe cells to cholesterol depletion, believed to disassemblethe rafts and to reveal therefore their role in specific processes.Interestingly, this treatment had been reported to inhibit alltypes of regulated exocytosis investigated so far (Lang et al.,2001; Ohara-Imaizumi et al., 2004; Salaun et al., 2004). InPC12-27 cells, depletion was amply effective, as revealed bythe blockade of the cholera toxin endocytosis. Also, the enlargeosomeswere affected, showing increased fragility, redistribution fromthe peripheral areas to the whole cytoplasm, formation of clumpsand vacuoles, accumulation of d/A at the surface of restingcells, possibly due to disturbance of the trafficking to and/orfrom the plasma membrane. However, the enlargeosome exocyticresponses induced by ionomycin were unchanged, suggesting theirpossible independence from the existence of rafts. After theinsensitivity to tetanus toxin, this seems to be another propertythat distinguishes the regulated exocytosis of enlargeosomesfrom those of other exocytic organelles.

The proposal of the enlargeosome as a new type of organellewas initially based on its distinction from the classical cytoplasmicstructures, the ER, Golgi complex, TGN, sorting and recyclingendosomes, lysosomes, glut4-rich vesicles, and constitutivesecretory vesicles. The detergent resistance of the enlargeosomemembrane opened now the possibility of a link to the other detergent-resistantorganelles, in particular to caveolin-rich vesicles, caveosomes,and other known raft-rich vesicles trafficking between the TGNand the plasma membrane. Of the three raft markers investigated,however, caveolin1 was found to lack any colocalization withd/A, whereas Thy1 and also flotillin1, which is localized notin a single type of membrane but is distributed to various types(Morrow et al., 2002; Kokubo et al., 2003), exhibited only alow degree of colocalization. These results exclude the identificationof enlargeosomes with organelles specific for the three markers.A considerable colocalization of d/A with flotillin1 becameapparent at the cell surface after stimulation of exocytosis.Because, however, the resolution of confocal images is low comparedwith the size of the raft microdomains, the significance ofthe observation, in particular whether it was due to real intermixingof the exocytized d/A-rich membrane domains with those richin flotillin1, remains to be established.

A property of the enlargeosome system that so far was completelyunknown is endocytosis. In the previous patch-clamp and immunocytochemicalstudies (Ninomiya et al., 1996; Kasai et al., 1999; Borgonovoet al., 2002; Cerny et al., 2004), the process had not beenspecifically investigated. Now, we have found that a low-rateendocytosis of d/A-rich patches occurs even in resting cells,presumably as a consequence of spontaneous enlargeosome exocyticevents, and that intense endocytosis follows the stimulation-inducedexocytic responses. Also in the stimulated cells, however, endocytosisis markedly asynchronous: it is appreciable within one or afew minutes from the stimulation only in a fraction of cells,whereas in others it requires longer times to become well appreciable.For obvious technical reasons, only the cells of the first groupcould be studied by both patch clamping and immunocytochemistry,whereas with the others only the second experimental approachcould be used.

Several aspects of the enlargeosome endocytosis are of interest.Among the PC12-27 cells investigated by patch clamping, thosethat responded to stimulation with [Ca²⁺]_i rises >4.5 µMexhibited capacitance decrease rates several-fold faster thanthose that had reached values <4 µM. The enlargeosomeendocytosis seems therefore to be regulated, a property that,in other cells and secretory systems, has already attractedgreat interest (Sankaranarayanan and Ryan, 2001; Sorkin andVon Zastrow, 2002; Maxfield and McGraw, 2004). Moreover, theintracellular vesicles positive for d/A maintained a neutralpH in their lumen. This result excludes the involvement of theendosomes generated from coated pits and vesicles, characterizedby their classical acidic lumen (Maxfield and McGraw, 2004);however, it seems insufficient for the identification of theorganelles involved. Various types of nonacidic endosomes havein fact been described, trafficking independently or coordinatelywith each other and with acidic endosomes along multiple intracellularpathways (Nichols and Lippincott-Schwartz, 2001; Nabi and Le,2003; Nichols, 2003; Parton and Richards, 2003; Massol et al.,2004). Finally, a sequence of the events occurring within 30min after the generation of the d/A-positive endocytic vesiclescould be deduced from the ultrastructural study of cells thathad internalized antibody in the course of ionomycin stimulation.Early vesicles, relatively small and moderately immunolabeled,developed into more heavily labeled organelles, i.e., largervesicles and then vacuoles with a few segregated vesicles intheir lumen and some vesicles budding from their cytosolic surface.Interestingly, the TGN seemed completely excluded from the d/A-positiveendocytic pathway. Further work is needed to investigate thenumerous issues still open in the field, in particular to identifythe nature of the d/A-positive endosomes, to map in more detailtheir intracellular pathway, and to clarify the possible roleof this recycling system in the regeneration of enlargeosomescompetent for regulated exocytosis

In conclusion, the enlargeosomes that emerge from the presentstudy are significantly more detailed than those known untilnow (Borgonovo et al., 2002). Working on the PC12-27 cell model,we have shown that this new type of vesicle does indeed participatein the regulated exocytic responses and does account, at leastin large part, for the surface enlargements revealed by patch-clampcapacitance, induced by both photolysis of caged Ca²⁺ compoundsand the Ca²⁺ ionophore ionomycin; that its membrane, resistantto nonionic detergents, is different from other membranes sharingthis property; that cholesterol extraction does not block itsexocytosis; and that after exocytosis its membrane is recycledby a nonacidic form of endocytosis. Enlargeosomes seem thereforeto have a specific profile, compatible with a wide role in physiologyand possibly also in pathology. In addition to their intrinsicinterest, these results promise to be instrumental for futurestudies on multiple aspects of the enlargeosome cell biologythat are still unknown, including the biogenesis and intracellulartransport of the organelles, the molecular mechanisms of theirexocytic membrane fusion, and the nature and pathways of theirendocytic system.

ACKNOWLEDGMENTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

We thank Erwin Neher for support, and Evelina Chieregatti andMichela Matteoli for suggestions and criticisms. This work wassupported by grants from the European Union (Growbeta n. QLG3-CT2001-02233and Apopis LSHM-CT-2003-503330), the Italian Ministero dell'Istruzione,dell'Università e della Ricerca (Cofin 2001 and 2002;FIRB), Telethon, and the Italian National Research Council (ConsiglioNazionale delle Ricerche: Physiopathology of the Nervous Systemand Functional Genomics). During part of the work, E.C. wasa European Union Marie Curie fellow at the European NeuroscienceInstitute (Göttingen, Germany).

Footnotes

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.E04–07–0577.Article and publication date are available at www.molbiolcell.org/cgi/doi/10.1091/mbc.E04–07–0577.

Abbreviations used: antibody, mouse monoclonal antibody raisedagainst d/A; [Ca²⁺]_i, cytosolic concentration of free calcium;cdx, methyl- ${beta}$ -cyclodextrin; d/A, desmoyokin/Ahnak; DG, densegranule; DM-nitrophen, dimethoxynitrophenamine tetrasodium salt;EEA1, early endosomal antigen 1; fF, femtoFarad, unit of capacitance;FITC, fluorescein isothiocyanate; TRITC, tetramethylrhodamineisothiocyanate; Lamp1, lysosomal membrane glycoprotein 1; NP-EGTA,o-nitrophenyl EGTA; PC12, rat pheochromocytoma cell line; SLMV,synaptic-like microvesicle; TeTx, tetanus toxin; TGN, trans-Golginetwork; TX-100, Triton X-100; wt, wild-type.

The online version of this article contains supplemental materialat MBC Online (http://www.molbiolcell.org).

Corresponding author. E-mail address: meldolesi.jacopo{at}hsr.it.

REFERENCES

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