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Previous Article | Next Article
The Journal of Neuroscience, April 1, 1999, 19(7):2464-2473
A Test of the Cytosolic Apolipoprotein E Hypothesis Fails to Detect the Escape of Apolipoprotein E from the Endocytic Pathway into the Cytosol and Shows that Direct Expression of Apolipoprotein E in the Cytosol is Cytotoxic
Ronald B. DeMattos, Fayanne E. Thorngate, and David L. Williams Department of Pharmacological Sciences, University Medical Center, State University of New York at Stony Brook, Stony Brook, New York 11794
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Genetic evidence indicates that apolipoprotein E4 (apoE4) is a risk factor for the development of Alzheimer's disease. A controversial hypothesis proposes that apoE, a typical secretory protein, accesses the neuronal cytosol in which apoE3, but not apoE4, protects tau from hyperphosphorylation. However, no conclusive evidence for the presence of apoE in the cytosolic compartment has been presented. We designed a novel assay to test whether apoE can access the cytosol via escape from the endocytic pathway by incorporating a nuclear localization signal (NLS) into apoE. Control experiments demonstrated that apoE plus NLS (apoE+NLS) is chaperoned to the nucleus if it reaches the cytosolic compartment. When exogenous apoE+NLS was endocytosed by neuronal cells, no nuclear apoE was detected, indicating that apoE remains within the endocytic pathway and does not escape into the cytosol. Furthermore, we show that direct cytosolic expression of apoE is cytotoxic. These data argue that effects of apoE on the neuronal cytoskeleton and on neurite outgrowth are not mediated via cytosolic interactions but rather by actions originating at the cell surface.
Key words: Alzheimer's disease; apoE; cytosolic; cytotoxic; endocytosis; microtubules; nuclear localization assay; tau
INTRODUCTION
Apolipoprotein E (apoE) is a secretory protein that plays a major role in cholesterol homeostasis in the plasma (Weisgraber, 1994
). ApoE is an atypical apolipoprotein in that it is produced by many extrahepatic tissues (Blue et al., 1983
There are three common isoforms of apoE arising from single amino acid interchanges at positions 112 and 158 (Zannis et al., 1982
4 allele of apoE has been identified as a risk factor for the development of late-onset familial and sporadic Alzheimer's disease (AD) (Rebeck et al., 1993
peptide to apoE (Strittmatter et al., 1993a
A model was proposed that links the apoE isoform-specific observations to the development of AD (Strittmatter et al., 1994b
In the present study, we developed a novel assay to determine the location of apoE within neuronal cells by using the nuclear localization pathway to distinguish between apoE that is enclosed by membranes (endosomal-lysosomal) or truly cytosolic. This protein sorting system has only two requirements: first, the protein that is to be transported to the nucleus must contain a recognizable nuclear localization signal (NLS), and second, the protein must be in the cytosol (Roberts et al., 1987
MATERIALS AND METHODS The establishment and characterization of an apoE expression vector series. Construction of expression vectors for wild-type and modified forms of apoE was accomplished by standard molecular cloning techniques. The four vectors shown in Table 1 were made using an apoE-specific PCR protocol, followed by replacement subcloning into the vectors pC1E3 and pC1E4 (DeMattos et al., 1998
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Table 1. Apolipoprotein E expression vectors Production and maintenance of stable apoE Neuro-2a cell lines. Neuro-2a cells were maintained in a 37°C humidified 95% air-5%CO2 incubator in medium A [DMEM/F-12 (1:1) supplemented with 10% heat-inactivated fetal bovine serum (FBS) (Atlanta Biologicals), 4 mM glutamine, 100 U/ml penicillin, 100 U/ml streptomycin sulfate, and 0.25 µg/ml amphotericin B]. Neuro-2a cells were plated at 1.0 × 106 cells in 10 ml of medium A per 10 cm dish and were transfected with 20 µg of plasmid using a standard calcium phosphate precipitation protocol (Chen and Okayama, 1987
Western blotting analysis. Cells were plated at 1.0 × 107 cells in 10 ml of medium A per 10 cm dish, incubated overnight at 37°C, washed twice with medium A, and incubated for an additional 24 hr in 10 ml of fresh medium A. Conditioned medium was removed, and cells were washed two times with PBS and solubilized in 0.5 ml of 2% SDS in PBS for total protein determination. Conditioned medium and cell lysates (100 µg) were run on a 10% polyacrylamide-SDS gel, electrophoretically transferred to nitrocellulose, and blocked for 1 hr at room temperature in TBS (20 mM Tris-HCl, pH 7.4, and 150 mM NaCl) containing 7% nonfat milk and 0.05% Tween 20. The blocked membrane was incubated with affinity-purified polyclonal goat anti-human apoE antibody (BioDesign International, Kennebunk, ME) at 2 µg/ml overnight at room temperature in TBS containing 1% nonfat milk and 0.2% Tween 20. The membrane was washed three times with TBS containing 0.05% Tween 20 and incubated with a horseradish peroxidase-conjugated anti-goat IgG (Sigma, St. Louis, MO) for 1 hr at room temperature in TBS containing 1% nonfat milk and 0.05% Tween 20. Bands were visualized by enhanced chemiluminescence (Amersham, Arlington Heights, IL).
Stable transfection efficiency assay. Stable transfection efficiencies were determined by transfecting 1.0 × 106 Neuro-2a cells in 10 cm dishes with 20 µg of plasmid coding for either secreted apoE or intracellular apoE. Stable integrants were selected for 9-12 d with 350 µg/ml G418 (Life Technologies). Plates were washed three times with PBS, and the cells were fixed with 2.5% glutaraldehyde, permeabilized with 1% Triton X-100, and stained with ethidium bromide. Images were collected with a UV transilluminator with a video camera attachment (Ultra-Violet Products, Upland, CA) and were saved as tagged image file format files. The number of cell colonies per image was determined with the UTHSCSA Image Tool program (developed at the University of Texas Health Science Center at San Antonio, Texas and available from the internet by anonymous file transfer protocol from ftp:maxrad6.uthscsa.edu) The experiment was repeated with three different plasmid preparations.
ApoE immunocytochemistry. Neuro-2a stable cell lines and transiently transfected cells were analyzed for apoE immunocytochemistry as described previously (DeMattos et al., 1998
Transient Neuro-2a transfections. Transient apoE expression for Western blot analysis was accomplished by transfecting 1.0 × 106 cells per 10 cm dish with 20 µg of plasmid and analyzing the cells after 12 hr for apoE expression. Neuro-2a cells were plated onto 18 mm glass circle coverslips in 12-well tissue culture plates at a density of 8.0 × 104 cells per well and were subsequently transfected with 1 µg of plasmid. After 12 hr of expression, the cells were analyzed by apoE immunocytochemistry.
ApoE and apoE+NLS isolation and association with lipids. Neuro-2a cells secreting either apoE or apoE+NLS were grown to confluence in T175 flasks. Serum free media (DMEM/F-12, 1:1) was conditioned for 24 hr for either cell line. The conditioned media was passed through a D100 weakly basic anion exchange filter (Satorius) and apoE eluted with 1 M ammonium bicarbonate. The eluted apoE was diluted 10-fold with sterile distilled water and recirculated over HiTrap heparin columns (Pharmacia, Piscataway, NJ). The heparin-bound apoE or apoE+NLS was eluted with 1 M ammonium bicarbonate. Fractions containing apoE were pooled and dialyzed against PBS (this fraction is referred to as lipid-poor apoE). ApoE dimyristoyl-phosphatidylcholine (Sigma) disks were prepared as described previously (Innerarity et al., 1979
The nuclear localization assay. Neuro-2a cells were plated at 1.0 × 106 cells per 60 mm dish in complete medium (DMEM/F-12, 1:1, plus 10% FBS). After 24 hr, the medium was changed to N2 medium [DMEM/F-12, 1:1, plus N2 growth supplements (Life Technologies) (Bottenstein and Sato, 1979
RESULTS The nuclear localization assay
The inherent limitations of immunocytochemical studies make it difficult to discern whether apoE observed in neurons is membrane-enclosed within the endosomal-lysosomal pathway or actually free in the cytosol. The nuclear localization assay allows us to characterize the intracellular location of apoE by using an active pathway that can only sort ligands to the nucleus if they are present in the cytosol. We constructed expression plasmids coding for wild-type apoE and for apoE+NLS by PCR. Wild-type apoE3 and apoE3+NLS proteins were secreted by cells, isolated from culture medium, and added to neuronal cells for subsequent localization studies.
The site in which an NLS is incorporated into a protein may effect its recognition. An NLS can function in a variety of sites within a protein, yet in some locations it may be masked (Roberts et al., 1987
SP) when expressed in cells. The second control plasmid also lacks a signal peptide but has a C-terminal NLS (apoE+NLS
Cytosolic apoE is toxic
Neuro-2a cells were transfected with the plasmids listed in Table 1 and selected for resistance to G418. The neomycin resistance gene is present in each of the plasmids. Three clonal cell lines for each plasmid were screened for apoE expression. Northern blot analysis of apoE3 mRNA (Fig. 1) and Western blot analysis (Fig. 2) confirmed that wild-type apoE3 and apoE3+NLS were expressed and that the proteins accumulated in the culture medium. We did not detect any apoE expression for either of the signal peptide bypass plasmids (apoE
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Figure 1. Northern blot of apoE mRNA in stably transfected cell lines. Total RNA (25 µg/lane) prepared from the indicated Neuro-2a cell lines was denatured and separated by electrophoresis on a 1.2% formaldehyde-agarose gel. After transfer to a nylon membrane, the RNA was visualized by ethidium bromide staining to verify that equal amounts of intact RNA were present (A). The membrane was probed with a 32P-labeled random primed apoE fragment (nucleotides 209-653), and hybridization was visualized with a Molecular Dynamics (Sunnyvale, CA) PhosphorImager (B).
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Figure 2. Western blot of apoE secreted by stably transfected cell lines. Conditioned medium (A) and cytoplasmic proteins (B) from the indicated cell lines (100 µg of protein/lane) were separated by 10% SDS-PAGE and were electroblotted to a nitrocellulose membrane. The membrane was probed with an affinity-purified polyclonal goat anti-human apoE antibody, and bands were visualized by enhanced chemiluminescence.
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Figure 3. Stable transfection efficiency assay. Neuro-2a cells were plated at a density of 1.0 × 106 per 10 cm dish and were calcium phosphate-transfected with 20 µg of plasmid for apoE3 or apoE3-SP. Control plates lacked the addition of plasmid DNA during the transfection protocol. Stable integrants were selected for 9-12 d with 350 µg/ml G418. The cells were then fixed in 2.5% glutaraldehyde, permeabilized with 1% Triton X-100, and stained with ethidium bromide. Cell colonies were visualized with a UV transilluminator, and images were captured with a video camera attachment. The number of transfectants per plate (each colony represents a single transfectant) is shown in the bottom right corner of each panel. The assay was repeated three times with three different plasmid preparations.
Analysis of cytosolic apoE in transient transfection assays
Expression of the signal peptide bypass plasmids was necessary to verify that the incorporated NLS is recognized if apoE enters the cytosolic compartment. Because stable expression of cytosolic apoE is toxic, we switched to a transient transfection assay to allow us to test for cytosolic apoE before it kills the cells. Neuro-2a cells transfected with plasmids coding for apoE3, apoE3
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Figure 4. Western blotting of Neuro-2a cells transiently expressing apoE plasmids. Neuro-2a cells were plated at a density of 1.0 × 106 per 10 cm dish and were transfected with 20 µg of plasmid for apoE3, apoE3-SP, or apoE3+NLS-SP. Cell lysates from transfected and control nontransfected Neuro-2a cells were prepared after 12 hr of expression. Cell lysates (100 µg) were analyzed for apoE by Western blotting as described in Materials and Methods.
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Figure 5. Immunocytochemical analysis of Neuro-2a cells transiently expressing apoE plasmids. Neuro-2a cells were analyzed by apoE immunocytochemistry after 12 hr of expression. Cells were transfected with apoE3 (A), apoE3-SP (B), or apoE3+NLS-SP (C). Neuro-2a cells (D) were also treated with a mock transfection (no plasmid). ApoE localization was detected with an affinity-purified polyclonal goat anti-human apoE antibody and a rhodamine-conjugated secondary antibody. All images were collected by confocal microscopy with a 60× oil immersion lens. Scale bars, 10 µm.
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Figure 6. Immunocytochemical analysis of nuclei isolated from Neuro-2a cells transiently expressing apoE plasmids. Neuro-2a cells were transfected with apoE3, apoE3-SP, or apoE+NLS-SP plasmids, and nuclei were isolated after 12 hr of expression. Nuclei were processed for apoE immunoreactivity as described in Materials and Methods. There are several hundred nuclei present in each of the three panels, yet only those nuclei that contain apoE are illuminated. Inset shows a high-magnification view of one of the apoE-positive nuclei isolated from Neuro-2a cells transiently expressing apoE3+NLS. The images were collected by confocal microscopy with a 20× objective. Scale bars, 50 µm. Inset was collected with a 60× oil immersion lens. Scale bar (in inset), 5 µm.
ApoE and apoE+NLS intracellular localization
We next tested whether apoE3 or apoE3+NLS is endocytosed when added to cells. ApoE3 and apoE3+NLS were isolated by a combination of anion exchange and heparin affinity chromatography from conditioned media of transfected Neuro-2a cells. ApoE3 isolated from these cell cultures was shown previously to be poorly lipidated (DeMattos et al., 1998
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Figure 7. Immunocytochemical localization of endocytosed apoE disks. ApoE3 and apoE3+NLS were isolated from conditioned media and recombined with dimyristoyl-phosphatidylcholine to form lipoprotein disks. Neuro-2a cells were incubated with lipoprotein disks for 4 hr, and the endocytosed apoE was identified by immunocytochemistry. Control cells lacked the addition of the apoE lipoproteins. ApoE localization was detected with an affinity-purified polyclonal goat anti-human apoE antibody and a rhodamine-conjugated secondary antibody. The endocytosed apoE appears to be highly localized within membrane vesicles in a perinuclear compartment that may be indicative of neuronal lysosomes (arrows). All images were collected by confocal microscopy with a 60× oil immersion lens. Scale bars, 20 µm.
Endocytosed apoE does not escape into the cytosol
Parental Neuro-2a cells were incubated in the presence of varying concentrations of apoE3 lipoproteins for 4 hr. After washing the cells and removing cell surface apoE by trypsin digestion, the cells were fractionated into cytoplasmic (all intracellular constituents except nuclei) and nuclear fractions. A sensitive ELISA was used to determine the apoE content of each fraction. The cytoplasmic fraction contained membrane-bound apoE (endosomal-lysosomal), whereas the nuclear fraction contained any apoE that escaped to the cytosol.
To ensure the repeatability of the nuclear localization assay, we performed two identical experiments on separate days with two independent apoE particle preparations (Table 2, experiments A, B). Neuro-2a cells in duplicate plates were incubated for 4 hr with either apoE3 or apoE3+NLS disks at a concentration of 10 µg/ml and were processed as described above. In both experiments, similar levels of apoE3 and apoE3+NLS were found in cytoplasmic extracts. There was minimal variation in endocytosis of apoE between particle preparations. No nuclear apoE was detected in either experiment, thereby indicating that no detectable apoE escaped the endocytic pathway. We analyzed the culture medium after the 4 hr incubation to determine the degree of apoE clearance. We observed substantial clearance of apoE3 and apoE3+NLS during the incubation period (an average of 42% of total apoE added was cleared). The clearance value (42%) is the sum of degraded apoE, extracellularly associated apoE, and apoE detected in the cell. Neuro-2a cells have been shown to have the capacity to degrade large quantities of lipoproteins during short incubation periods (Bellosta et al., 1995
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Table 2. Apolipoprotein E nuclear localization assay We next tested whether increasing particle uptake would result in cytosolic apoE. Neuro-2a cells were incubated with 25 µg/ml apoE3 or apoE3+NLS disks, and the subcellular location of the endocytosed apoE was determined (Table 2, experiment C). Although there was a fivefold increase in the amount of apoE found within the cytoplasmic extracts, nuclear apoE was not detected. Because lipoprotein uptake has been reported to be enhanced by the addition of lipid-free apoE (Ji et al., 1998
We next asked whether the use of different endocytic pathways could result in the escape of apoE to the cytosol. Because lipoprotein size has been shown to be a determining factor for receptor specificity (Tabas et al., 1991
< 1.006). The purified particles were then used in our standard 4 hr nuclear localization assay at a concentration of 10 µg/ml (apoE). ApoE3-
DISCUSSION Determining the validity of the cytosolic apoE hypothesis is critical for evaluating the physiological significance of apoE-tau interactions and understanding the risk factor association of apoE and Alzheimer's disease (Strittmatter et al., 1994b
We used transient transfection and expression of the signal peptide bypass plasmids to verify that the cell recognizes the NLS in apoE. Immunocytochemical results demonstrate that the incorporated NLS was recognized, because the apoE3+NLS was actively chaperoned to the nuclei of Neuro-2a cells. Additionally, we showed that the diffuse cytosolic staining pattern of apoE3
Our sensitive nuclear localization assay demonstrates that apoE does not appear to escape the endocytic pathway at a detectable level in a neuroblastoma cell line. This assay quantitatively measures the subcellular localization of endocytosed apoE and apoE+NLS. A murine neuroblastoma cell line (Neuro-2a) was used for these experiments because our group and others have shown previously that the Neuro-2a cells exhibit apoE isoform-specific differences in neurite outgrowth (Bellosta et al., 1995
The sensitivity of the nuclear localization assay is determined by two factors: the overall amount of apoE endocytosed and the sensitivity of detection of apoE within the nuclear fraction. The ELISA can readily detect 5 ng of apoE/mg of cell protein. Based on these considerations, the sensitivity for detecting apoE in the nuclear fraction can be assessed in two ways. In the first, the detection limit can be compared with the steady-state level of apoE within the cell. For example, in Table 2, experiments A, B, C, and D, the assay could have detected 3.5, 3.5, 0.7, and 3%, respectively, of the steady-state apoE within the cell. By this measurement, if as little as 0.7% of the apoE within the endocytic pathway had escaped to the cytosol (experiment C), it could have been detected in the nuclear fraction. The sensitivity would have been less in experiments E and F because of the lower levels of cellular apoE.
In the second, the detection limit can be compared with the amount of apoE cleared from the medium, which is a reflection of the cumulative amount of apoE processed by the endocytic pathway during the assay. Because our assay procedure removed cell surface and extracellular matrix apoE by trypsin treatment, the values for apoE clearance from the medium must be corrected for these factors. Using the very conservative estimate that only 15% of the cleared apoE was processed and degraded by the endosomal-lysosomal pathway in the 4 hr assay with Neuro-2a cells (Bellosta et al., 1995
Our final experiments indicate that, regardless of the endocytic receptor system targeted, apoE does not escape into the cytosol. Preliminary Western blot studies indicate that Neuro-2a cells express the low-density lipoprotein receptor, the very low-density lipoprotein receptor, and the low-density lipoprotein receptor-related protein (R. B. DeMattos, D. K. Strickland, and D. L. Williams, unpublished observations); further studies will determine whether Neuro-2a cells express other members of the LDL receptor super family. We performed nuclear localization experiments with apoE3 or apoE3+NLS that were associated with
Our results demonstrate that the vast majority of endocytosed apoE does not gain access to the cytosolic compartment of Neuro-2a cells. It is important to note that the Neuro-2a cells have been shown by two independent groups to develop apoE isoform-specific neurite outgrowth differences under the same culture conditions as in this study. These results indicate that the isoform-specific stimulation of neurite outgrowth is unlikely to be caused by apoE in the cytosol. More likely, apoE alters neurite outgrowth via an unknown isoform-specific mechanism originating at the cell surface. Possible mechanisms could be receptor-mediated signaling cascades or an apoE-dependent cell matrix adhesion event. There is suggestive evidence for each of these possibilities in the literature (Misra et al., 1994
FOOTNOTES Received Nov. 17, 1998; revised Jan. 11, 1999; accepted Jan. 19, 1999.
This work was supported by National Institutes of Health, National Heart, Lung, and Blood Institute Grant HL 32868. R.B.D. was partially supported by a predoctoral fellowship from the Institute for Cell and Developmental Biology, State University of New York at Stony Brook. F.E.T. was partially supported by Institutional National Research Award IT32-DK-07521. We thank Miguel Berrios and William Theurkauf for advice on confocal microscopy and Joel Levine for helpful discussion.
Correspondence should be addressed to David L. Williams, Department of Pharmacological Sciences, University Medical Center, State University of New York at Stony Brook, Stony Brook, NY 11794.
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