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© The Rockefeller University Press,
0021-9525/2001//1511 $5.00
The Journal of Cell Biology, Volume 153, Number 7,
, 2001 1511-1518
Report |
Nucleocytoplasmic Shuttling of Endocytic Proteins
pdifiore{at}ieo.it
Many cellular processes rely on the ordered assembly of macromolecular structures. Here, we uncover an unexpected link between two such processes, endocytosis and transcription. Many endocytic proteins, including eps15, epsin1, the clathrin assembly lymphoid myeloid leukemia (CALM), and
-adaptin, accumulate in the nucleus when nuclear export is inhibited. Endocytosis and nucleocytoplasmic shuttling of endocytic proteins are apparently independent processes, since inhibition of endocytosis did not appreciably alter nuclear translocation of endocytic proteins, and blockade of nuclear export did not change the initial rate of endocytosis. In the nucleus, eps15 and CALM acted as positive modulators of transcription in a GAL4-based transactivation assay, thus raising the intriguing possibility that some endocytic proteins play a direct or indirect role in transcriptional regulation.
Key Words: endocytosis • nucleocytoplasmic shuttling • eps15 • CRM1 • transcription
© 2001 The Rockefeller University Press
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Introduction |
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 TopAbstract Introduction Materials and MethodsResults and DiscussionReferences |
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The major nuclear export pathway relies on the interaction between NES-containing proteins and the chromosomal region maintenance protein (CRM)1/exportin1 receptor (Fornerod et al. 1997; Fukuda et al. 1997; Ossareh-Nazari et al. 1997; Stade et al. 1997). The small GTPase Ran in its active form (Ran-GTP) is absolutely required for this interaction. By cooperatively binding to CRM1 in the presence of NES-containing cargo molecules, Ran-GTP allows the formation of a trimeric Ran-GTP–CRM1–NES complex (Fornerod et al. 1997; Izaurralde et al. 1997). The antifungal antibiotic leptomycin B (LMB) specifically inhibits CRM1 (Kudo et al. 1998). By selectively modifying a single cysteine residue in CRM1 (Kudo et al. 1999), LMB interferes with the formation of RanGTP–CRM1–NES complexes, leading to nuclear accumulation of NES-containing proteins (Askjaer et al. 1998). Thus, LMB has represented a powerful tool to investigate nuclear shuttling of several proteins. More interestingly, LMB has allowed the unexpected detection of nuclear translocation of a variety of proteins with predominant extranuclear localization and function, such as the membrane-associated guanylate kinase CASK/LIN-2 (Hsueh et al. 2000), LIM-containing lipora-preferred partner (an actin cytoskeleton protein) (Petit et al. 2000), and actin (Wada et al. 1998). Therefore, it is predicted that LMB-aided analysis will unveil more nuclear translocation events of proteins whose export rate is too high to determine substantial nuclear accumulation at steady state.
Endocytic proteins might constitute one such class of molecules. Scattered evidence supports the idea that the molecular machinery of endocytosis might also play some currently undefined function in the nucleus. Box-dependent myc-interacting protein-1, which is related to amphiphysin, displays nuclear localization (Sakamuro et al. 1996). Eps15R, a bona fide endocytic protein, also shows a dual cytosolic/nuclear distribution (Coda et al. 1998). Epsin1, another endocytic protein, accumulates in the nucleus in the presence of LMB when overexpressed (Hyman et al. 2000). Functional evidence linking endocytic proteins to nucleocytosolic transport also exists as shown by findings that eps15 and eps15R play a role in the CRM1-based nuclear export pathway (Doria et al. 1999).
A major argument against a hypothetical function in the nucleus is that, by and large, endocytic proteins do not display nuclear localization. However, this might be due to a high rate of nuclear export. In this study, we undertook a systematic analysis of the subcellular distribution of several endocytic proteins under conditions of blockade of nuclear export as obtained by LMB treatment. Surprisingly, we found that several of the analyzed proteins accumulate in the nucleus under these conditions, thus indicating nucleocytoplasmic shuttling of endocytic machinery. In the nucleus, two endocytic proteins, eps15 and CALM, acted as transcriptional modulators in a GAL4-based transactivation assay. Our results uncover an unexpected property of several endocytic proteins and suggest their participation in nuclear events, possibly including regulation of transcription.
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Materials and Methods |
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TopAbstractIntroductionMaterials and MethodsResults and DiscussionReferences |
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-adaptin (AP.6; Affinity BioReagents, Inc.), anti–
-adaptin and –β-adaptin (100/3 and 100/1, respectively; Sigma-Aldrich), anti–µ2-adaptin (AP50; Transduction Laboratories), anti-clathrin (X22; provided by T. Kirchhausen, Harvard Medical School, Boston, MA), polyclonals anti-CALM (C-18; Santa Cruz Biotechnology, Inc.), anti-dynamin II (C-18; Santa Cruz Biotechnology, Inc.), anti-epsin1 (R-20; Santa Cruz Biotechnology, Inc.), and anti-rab5 (provided by M. Zerial, Max-Planck Institute, Dresden, Germany). Alexa red and green secondary antibodies (Molecular Probes) were used. Images were acquired using a confocal 1024MRC Bio-Rad Laboratories microscope equipped with a krypton-argon laser.
A semiquantitative analysis of the experiment shown in Fig. 3 B was performed with the NIH Image software by measuring the pixel density in the nucleus relative to the cytosol on central sections obtained by confocal microscopy. Values were obtained for five cells for each experimental condition. Results, expressed as the cytosol/nucleus ratio for each protein, were (the first value refers to untransfected cells, the second to rab5S34N-transfected cells): eps15, 3.4, 3.8; CALM, 5.6, 5.0; epsin, 4.7, 4.1; -adaptin, 2.6, 3.0. SD was <20% of the mean in all cases.
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Internalization Assays
Internalization assays using fluorochrome-conjugated ligands have been described previously (Lanzetti et al. 2000). For internalization experiments using radiolabeled ligands, HeLa cells grown in 6-well dishes were serum starved for 3 h before the addition of 2 ng/ml of 125I-EGF or 1 µg/ml of 125I-transferrin (Tf) in binding medium (DME with 20 mM Hepes, pH 7.4, and 0.1% BSA) for 2, 4, and 6 min at 37°C. The amount of surface-bound and internalized radioactivity was determined as previously described (Sorkin et al. 1993). The rate of internalization is expressed as the ratio between internalized and surface 125I-ligand for each time point. A low concentration of 125I-EGF was used to avoid saturation of the internalization machinery. Specific binding is reported for all data points. Nonspecific binding was measured by adding a 100-fold excess of cold EGF.
Luciferase Reporter Assays
For transcriptional assays, epsin1, CALM, eps15, and its truncated versions were cloned into the PM2 vector (Sadowski et al. 1992) fused to the GAL4 DNA-binding domain (amino acids positions 1–147). COS-7 cells grown in 6-well dishes were transiently transfected in triplicate with 0.3 µg of the GAL4-TK-luciferase reporter (provided by K. Helin, European Institute of Oncology, Milan, Italy) and with 1.2 µg of the different GAL4 fusion constructs using lipofectamine (Life Technologies). Cells were lysed after 48 h and analyzed by immunoblotting with anti-GAL4 antibodies (Santa Cruz Biotechnology, Inc.) to verify the levels of expression of the various GAL4 fusion proteins. Transactivation assays were then performed only on sets of transfectants that showed comparable levels of expression of the various proteins. Luciferase activity was measured on identical amounts of total cellular lysates from the various transfectants using a commercial kit (Promega).
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Results and Discussion |
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TopAbstractIntroductionMaterials and MethodsResults and DiscussionReferences |
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-adaptin, epsin1, and CALM (Fig. 1), whereas the distribution of clathrin, dynamin II, β-adaptin, µ2-adaptin, and -adaptin remained unchanged (Fig. 1). We note that in all cases the size of the shuttling endocytic proteins is above the cut-off value for free diffusion into the nucleus, which is 
50 kD.
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20–30%) shuttled in a CRM1-dependent manner as witnessed by the fact that we could never observe a dramatic depletion of the extranuclear pool (Fig. 1) even when higher doses and longer times of treatment with LMB were used (data not shown). The sum of our results indicates that endocytic proteins shuttle in and out of the nucleus and are exported through binding to CRM1.
Endocytosis and Nucleocytoplasmic Shuttling of Endocytic Proteins Are Independently Regulated Processes
We next investigated the reciprocal relationships between endocytosis and nucleocytoplasmic shuttling of endocytic proteins. Initially, we inhibited endocytosis and studied nuclear accumulation of endocytic proteins in the presence of LMB. A dominant negative mutant of rab5 (rab5S34N) (Lanzetti et al. 2000), which blocked endocytosis of both Tf and EGF receptors (Fig. 3 A), was transfected into CV-1 cells. Inhibition of endocytosis did not appreciably affect the nuclear accumulation of endocytic proteins (Fig. 3 B; a semiquantitative analysis is reported in Materials and Methods).
In a second set of experiments, we treated CV-1 cells with LMB for 16 h, a condition under which nuclear export is completely blocked, and then measured the uptake of radiolabeled ligands. As shown in Fig. 3 C, the initial rate of internalization of EGF and Tf was comparable in the presence or absence of LMB. Thus, endocytosis and nucleocytoplasmic shuttling of endocytic proteins are apparently independent processes.
Nucleocytoplasmic Shuttling of eps15 Is Not Regulated by Several Signaling Pathways
Nucleocytoplasmic transport is regulated frequently by signaling pathways. For example, nuclear shuttling of signal transducer and activator of transcriptions, the Net transcriptional repressor, and actin are regulated by tyrosine phosphorylation, UV/heat shock, and heat shock, respectively (Wada et al. 1998; Ducret et al. 1999; Milocco et al. 1999). Eps15 is tyrosine phosphorylated by active EGF receptors (Fazioli et al. 1993); thus, we employed it as a model to study the possible regulation of shuttling of endocytic proteins by signaling pathways.
Initially, we compared the nuclear accumulation of a mutant eps15 (FLAG-Y850F) in which the tyrosine phosphorylation site was mutagenized to Phe (Confalonieri et al. 2000) with that of a comparable wild-type construct (FLAG-eps15). Both the wild-type and mutant eps15 were clearly detectable in the nucleus upon LMB treatment (Fig. 4 A). Notably, wild-type eps15 accumulated in the nucleus upon LMB treatment even under serum starvation conditions (Fig. 4 A). In addition, EGF, serum, and phorbol ester treatment did not cause a significant increase in nuclear accumulation of eps15 (Fig. 4 B). Similarly, various stress-inducing stimuli, including UV, H2O2, and heat shock, did not appreciably change the partitioning of eps15 between the cytosol and the nucleus (Fig. 4 B). Finally, no appreciable changes in the nuclear accumulation of eps15 were evident even when the various stimuli were applied in the presence of LMB when compared with treatment with the inhibitor alone (data not shown). Thus, at least in the case of eps15, nucleocytoplasmic shuttling appears to be a constitutive process, which is not regulated by major signaling pathways.
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EH) were equally active, whereas a construct harboring the eps15 homology (EH) domains alone (GAL4-EH) or a mutant lacking the entire DPF region (GAL4-EH+coil) displayed no activity (Fig. 5 B). Thus, determinants contained in the COOH-terminal region of eps15 appear necessary for its effect on transcriptional regulation. Finally, deletion of the eps15 NES sequence (GAL4-858) resulted in a partial nuclear accumulation of this fusion protein at steady-state (data not shown) and in supertransactivation of the GAL4 promoter when compared with wild-type eps15 (Fig. 5 B).
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However, two lines of evidence suggest additional hypotheses. First, no immediate relationship between endocytosis and nucleocytoplasmic shuttling could be experimentally evidenced. Second, nuclear translocation of endocytic proteins was not influenced by several signaling stimuli, suggesting participation of these proteins in "basic" nuclear functions. Such a function could be transcription as witnessed by stimulation of transcription originating from a model promoter for two of the three endocytic proteins tested. We note that endocytic proteins contain multiple protein–protein interaction surfaces and are endowed with self-assembling properties (Marsh and McMahon 1999). Both endocytosis and transcription rely on the assembly of macromolecular scaffolds (Marsh and McMahon 1999; Lemon and Tjian 2000). Thus, it is tempting to speculate that the endocytic machinery functions in the nucleus as a whole, possibly by providing scaffold structures, which modify nuclear localization of specific transcription factors thereby regulating their function.
Our results might have important implications for the process of leukemogenesis. In acute myeloid leukemias, chromosomal translocations led to the formation of fusion proteins, frequently involving transcriptional regulators (Tenen et al. 1997). The emerging paradigm is that fusion proteins alter the subnuclear distribution of the transcriptional regulators involved, leading to subversion of the ordered series of transcriptional events required in the normal control of cell proliferation (Tenen et al. 1997). Endocytic proteins (eps15, CALM, and EEN) are also partners of fusion proteins in acute myeloid leukemia (Floyd and De Camilli 1998): a finding so far that could not be rationalized, given current theories. On the basis of our results, a unifying scenario can be proposed in which endocytic proteins participate to leukemogenesis by mislocalizing transcription factors and thus lead to transcriptional deregulation.
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Acknowledgments |
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This work was supported by grants from Associazione Italiana Ricerca sul Cancro, Telethon Italy (D-90), Istituto Superiore di Sanitá (AIDS 1999) and Centro Nazionale Ricerche (target project Biotechnology) to P.P. Di Fiore, and the Association pour la Recherche contre le Cancer (5807) to A. Benmerah.
M. Vecchi, J.W. van de Loo, and V. Poupon were supported by fellowships from Fondazione Italiana Ricerca sul Cancro, European Community (Marie Curie fellowship), and the Ligue Nationale contre le Cancer (Claude Bernard grant), respectively.
Submitted: 26 January 2001
Revised: 27 April 2001
Accepted: 9 May 2001
M. Vecchi and S. Polo contributed equally to this work.
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