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The Journal of Neuroscience, June 9, 2004, 24(23):5315-5321; doi:10.1523/JNEUROSCI.0913-04.2004

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Neurobiology of Disease
Estrogen and Androgen Protection of Human Neurons against Intracellular Amyloid _1-42 Toxicity through Heat Shock Protein 70

Yan Zhang,^1,4 Nathalie Champagne,⁴ Lenore K. Beitel,⁴ Cynthia G. Goodyer,² Mark Trifiro,^3,4 and Andréa LeBlanc^1,4

Departments of ¹Neurology and Neurosurgery, ²Pediatrics, and ³Human Genetics, McGill University, Montréal QB H3A 1B1, Canada, and ⁴The Bloomfield Center for Research in Aging, Lady Davis Institute for Medical Research, Jewish General Hospital, Montréal QB H3T 1E2, Canada

	Abstract

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Intracellular amyloid peptide (iA_1-42) accumulates in the Alzheimer's disease brain before plaque and tangle formation (Gouras et al., 2000) and is extremely toxic to human neurons (Zhang et al., 2002). Here, we investigated whether androgen and estrogen could prevent iA_1-42 toxicity, because both these hormones have a wide range of neuroprotective actions. At physiological concentrations, 17--estradiol, testosterone, and methyl testosterone reduce iA_1-42-induced cell death by 50% in neurons treated after the injection and by 80-90% in neurons treated 1 hr before the injection. The neuroprotective action of the hormones is mediated by receptors, because the estrogen receptor (ER) antagonist tamoxifen and the androgen receptor (AR) antagonist flutamide completely block the estrogen- and androgen-mediated neuroprotection, respectively. Transcriptional activity is required for the neuroprotective action, because dominant negative forms of the receptors that block the transcriptional activity of the ER and AR prevent estrogen- and androgen-mediated neuroprotection. Proteomics followed by Western blot analyses identified increased levels of heat shock protein 70 (Hsp70) in testosterone- and estrogen-treated human neurons. Comicroinjection of Hsp70 with the iA_1-42 blocks the toxicity of iA_1-42. We conclude that estrogen and androgens protect human neurons against iA_1-42 toxicity by increasing the levels of Hsp70 in the neurons.

Key words: intracellular amyloid; estrogen; androgen; neuroprotection; human neurons; Hsp70

	Introduction

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Intracellular amyloid _1-42 (iA_1-42) accumulates in the hippocampus and the entorhinal cortex neurons of mildly cognitively impaired and Alzheimer's disease (AD) individuals (Gouras et al., 2000; D'Andrea et al., 2001, 2002; Takahashi et al., 2002), in Down's syndrome brain neurons (Gyure et al., 2001; Busciglio et al., 2002), and in inclusion body myositis muscle cells (Querfurth et al., 2001; Sugarman et al., 2002). In AD, the accumulation of iA_1-42 precedes amyloid plaque formation (Gouras et al., 2000; D'Andrea et al., 2001). Cytosolically microinjected A_1-42 is selectively and highly toxic to human neurons in primary cultures (Zhang et al., 2002). In vivo, neuronal cytosolic A_1-42 transgenic expression induces neuronal loss in the cerebral cortex, hippocampus, and thalamus (LaFerla et al., 1995). Together, these results suggest that the accumulation of iA_1-42 is an early event in AD that could result in the dysfunction and eventual loss of neurons. Therefore, it is of interest to find inhibitors of intracellular A_1-42-mediated toxicity that may be useful as an early treatment in AD patients. In the present manuscript, we investigate the potential of androgens and estrogens as inhibitors of intracellular A_1-42-mediated toxicity in human neurons.

Despite controversy in vivo, there is strong evidence that both estrogens and androgens are neuroprotective in cell culture. Testosterone protects primary human neurons against serum deprivation (Hammond et al., 2001), cultured rat hippocampal neurons against extracellular A toxicity (Pike, 2001), rat neurons against heat shock-mediated hyperphosphorylation of tau by modulating glycogen synthase kinase 3 activation (Papasozomenos and Shanavas, 2002), cerebellar granule neurons against oxidative stress (Ahlbom et al., 1999, 2001), and rat hippocampal neurons against kainic acid-induced toxicity (Ramsden et al., 2003); testosterone also promotes neuritic extension in pheochromocytoma 12 cells (Lustig et al., 1994). Testosterone can protect through the androgen receptor (AR) rather than through aromatization into estrogen (Ahlbom et al., 2001; Hammond et al., 2001; Ramsden et al., 2003). Estrogen prevents caspase-6-mediated human neuronal cell death (Zhang et al., 2001), decreases A toxicity in cultured rat primary hippocampal neurons and human neuroblastoma SK-N-SH cells (Goodman et al., 1996; Green et al., 1996; Pike, 1999), inhibits serum deprivation-induced cell death in SK-N-SH cells (Goodman et al., 1996; Green et al., 1997), and protects against oxidative stress in mouse hippocampal neurons and neuronal injury induced by hemoglobin, chemical hypoxia, and excitatory amino acids (Behl et al.,1995, 1997). These steroid sex hormones can protect through activation of transcriptional activity or via signaling of survival pathways (Driggers and Segars, 2002; Heinlein and Chang, 2002; Segars and Driggers, 2002).

In the present study, we demonstrate that physiological concentrations of androgens or estrogens completely protect human neurons in primary cultures against microinjected iA_1-42 toxicity. Using AR and estrogen receptor (ER) antagonists and dominant negative forms of these receptors, we show that the neuroprotection occurs in a receptor- and transcription-dependent manner. Proteomics studies followed by Western blotting identify an increase in heat shock protein 70 (Hsp70) levels in testosterone- and estrogen-treated neurons. Hsp70 comicroinjected with iA_1-42 also completely prevents iA_1-42 toxicity. We conclude that testosterone and estrogen can protect against iA_1-42 through Hsp70.

	Materials and Methods

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A peptides, recombinant proteins, antibodies, and cDNAs
A peptides (Bachem, King of Prussia, PA) were dissolved in sterile distilled water at 25 µM and incubated at 37°C for 5 d (Zhang et al., 2002). The peptide stock solutions were kept frozen in aliquots until use. The recombinant human Hsp70 protein and monoclonal anti-Hsp70 antibody were purchased from Stressgen Biotech (Victoria, British Columbia, Canada). The wild-type and mutant 12474 and 15579 human androgen receptor cDNAs have been described previously. The AR mutants, 12474 and 15579, contain a deletion of 579Val and 580Phe and of 614Cys and 615Arg in the DNA binding domain (DBD), respectively (Beitel et al., 1994). All cDNAs were cloned into the vector pcDNA3 under the cytomegalovirus promoter (Panet-Raymond et al., 2000). The human ER wild-type and mutant DBD cDNAs were obtained from Dr. Sylvie Mader (University of Montreal, Montreal, Quebec, Canada). The DBD ER construct contains a deletion of amino acids 185-251 (Mader et al., 1993). All ER cDNAs were cloned into the pSG5 vector under the simian virus 40 promoter (Rosenauer et al., 1998). The androgen responsive element (ARE) luciferase reporter vector pGL3-MMTV-(ARE)-Luc and the estrogen responsive element (ERE) luciferase reporter vector pGL3-(ERE)-Luc have been described previously (Panet-Raymond et al., 2000). The cDNAs were purified with the UltraClean-15 DNA Purification kit (MoBio Laboratories Inc., Solana Beach, CA).

Human primary cell cultures and treatments
Primary cultures. Primary cultures of human neurons were prepared from 12- to 16-week-old fetal brains collected as approved by the McGill University Institutional Review Board and according to Canadian Institute of Health Research regulations (LeBlanc, 1995). In brief, fetal cortical brain tissues were dissected free of meninges and blood vessels in PBS (in M: 0.14 NaCl, 0.003 KCl, 0.01 Na₂HPO₄, and 0.002 KH₂PO₄, pH 7.2) and dissociated with 0.25% trypsin (Invitrogen, Burlington, Ontario, Canada). The trypsin was inactivated with 10% decomplemented fetal bovine serum (FBS; HyClone, Logan, UT), and released DNA was removed with DNase I (0.1 mg/ml; Sigma, Oakville, Ontario, Canada). The cells were filtered successively through 130 and 70 µm sterilized filters, washed with PBS, and washed with minimal essential medium (MEM) with Earle's balanced salt solution containing 0.225% sodium bicarbonate, 1 mM sodium pyruvate, 2 mM L-glutamine, 0.1% dextrose, 1x antibiotic Pen-Strep (all from Invitrogen), and 5% decomplemented FBS. Cells were then plated on poly-L-lysine-coated plates, flasks, or Aclar coverslips (33°C, 5 mm; Allied Chemical Inc., Minneapolis, MN) at a density of 3 x 10⁶ cells/ml. The cultures were incubated at 37°C with 5% CO₂, and the medium was changed every 48 hr. The neurons attached within 24 hr and developed extensive neuritic extensions within 3 d of plating. In general, the cultures contained 90-95% neurons and 5-10% astrocytes (LeBlanc, 1995).

Microinjection of A peptides and cDNA constructs in primary cultures of human neurons. Microinjections were performed 11 d after plating the neurons with the Eppendorf (Fishers, NY) Microinjector 5246 and the three-dimensional Burleigh (Fishers, NY) Micromanipulator MIS-5000 (Zhang et al., 2002). Microinjections were performed with a glass needle with a tip diameter of 0.5 µm pulled from 1.0 mm outer diameter and 0.5 mm inner diameter thin-walled glass capillaries with microfilament (borosilicate with filament MTW100F-4; World Precision Instruments, Sarasota, FL) with a Flaming/Brown micropipette puller (model P-87; Sutter Instruments, Novato, CA). Human neurons were injected at an injection pressure of 100 hPa, a compensation pressure of 50 hPa, and an injection time of 0.1 sec. The injected volume was 25 pl. A (10 nM), cDNAs (30 ng/ml), and Hsp70 (5 µg/ml) were coinjected with 100 µg/ml fluorescent marker dye Dextran Texas Red (DTR) (MW3000; Molecular Probes, Eugene, OR) into the cytosolic area of the neuron (Zhang et al., 2002). Approximately 90% of neurons survived the injection. Microinjections were done in 200 neurons per preparation in three independent neuron preparations, for a total of 600 injected neurons.

Treatment of human neurons with estrogen, androgen, tamoxifen, or flutamide. 17--Estradiol, 17--estradiol, BSA-17--estradiol, testosterone enanthate, and epitestosterone were purchased from Sigma. Methyl testosterone was bought from Pharmacopeia (Rockville, MD). Hormones were dissolved in 100% ethanol at a 5 mM concentration and diluted to 2-10 nM with culture medium before use (Hammond et al., 2001). Tamoxifen (TMX; Sigma) and flutamide (Flut; Sigma) were dissolved in sterile distilled water at 10 and 20 mM and serially diluted to the indicated concentration (2-10 nM) with MEM before treatment of neurons (Hammond et al., 2001). For the postincubation experiments, cells were microinjected with peptides or cDNAs and incubated at 37°C with hormones in the presence or absence of hormone receptor antagonists for 24 hr. For the preincubation experiments, cells were incubated at 37°C with hormones and hormone receptor antagonists for 1 hr before the microinjection of peptide followed by incubation with hormones in the presence or absence of hormone receptor antagonists for 24 hr.

Proteomics analyses and Western blot. Neurons were treated with 10 nM testosterone for 1 hr. The cells were washed in 1x PBS and collected in 10 mM Tris-HCl, pH 7.4, and 5 mM MgCl₂ for two-dimensional gel analysis. Cells were lysed with two freeze-thaw cycles in liquid nitrogen and extracts treated with 1000 U of DNase (Promega, Madison, WI) and 60 µg of RNase A for 10 min on ice. Proteins were precipitated with methanol-chloroform and solubilized in 9.5 M urea, 2.8% 3-[(3-cholamido-propyl)dimethylammonio]-1-propanesulfonate, 20 mM Tris-Cl, pH 7.4, 50 mM DTT, bromophenol blue, and 1% immobilized pH gradient buffer (Amersham Biosciences, Quebec, Canada). Proteins (100 µg) were separated by isoelectric focusing on IPGPhor IEF-13 cm strips (Amersham Biosciences). After isoelectric focusing separation, the gel strips were equilibrated with 50 mM Tris-Cl, pH 8.8, 6 M urea, 30% glycerol, 2% SDS, and 65 mM DTT buffer and placed on a 10% SDS-polyacrylamide gel for protein separation. The separated proteins were visualized by silver staining compatible with mass spectrometric analysis (Yan et al., 2000). Proteins that increased or decreased compared with untreated neurons were sent for mass spectrometric analysis at the Southern Alberta Mass Spectrometry Center in Calgary, Canada. To confirm increased levels of Hsp70 in human neurons exposed to estrogen and testosterone, 30 µg of proteins extracted from neurons treated with 10 nM estrogen or testosterone for 6 hr were immunoblotted with the monoclonal Hsp70 antibody, and the immunoreactivity was revealed with ECL.

Cell line cultures and treatments
MCF-7 and AR24 cell cultures. Human breast cancer MCF-7 cells (American Type Culture Collection, Manassas, VA) were cultured in RPMI 1640 medium (Invitrogen) with 10% FBS. AR24 cells were created by stably expressing human androgen receptors in rat motor neuron hybrid cells and cultured in DMEM (Invitrogen) with 5% FBS (Brooks et al., 1998). Cells were incubated at 37°C with 5% CO₂. The culture media was changed every 48 hr.

Transfection of MCF-7 and AR24 cells. Eighty percent confluent MCF-7 and AR24 cell cultures were washed and incubated at 37°C for 6 hr with 3 µg/ml cDNA and 6 µg/ml Lipofectamine-2000 (Invitrogen) in OPTIMEM (Invitrogen) without FBS. After the incubation, the cells were washed with DMEM-5% FBS and incubated at 37°C for 24 hr in the presence or absence of 10 nM estrogen or androgen.

Luciferase reporter system is used to measure androgen and estrogen receptor activity. The Dual-Luciferase Reporter Assay System kit (E1910; Promega) was used to investigate the dominant negative effects of the mutant AR and ER. The constructs with the firefly (Photnus pyralis) luciferase gene downstream of the ERE or ARE [pGL3-MMTV-(ARE)-Luc and pGL3-(ERE)-Luc] were cotransfected with the wild-type or mutant ER or AR constructs into estrogen receptor-positive MCF-7 or androgen receptor-positive AR24 cells, respectively. After treatment with 10 nM estrogen or testosterone, firefly luminescence was detected as indicated by the manufacturer. To control for transfection efficiency, the Renilla reniformis luciferase construct was cotransfected into cells. The activity was corrected for the protein concentration of each sample and expressed as [(firefly/renilla luciferase) x 10,000]. The luminescence is expressed as relative light units.

Measurement of cell death. Cells were fixed in fresh 4% paraformaldehyde and 4% sucrose in PBS for 20 min at room temperature and permeabilized in 0.1% Triton X-100 and 0.1% sodium citrate in PBS for 2 min on ice. Terminal deoxynucleotidyl transferase-mediated biotinylated UTP nick end labeling (TUNEL) was performed using the In Situ Cell Death Detection Kit I as described by the manufacturer (Roche, Quebec, Canada). The TUNEL-stained coverslips were then washed once in distilled water for 5 min and mounted on glass slides. The percentage of cell death was determined by the ratio of the number of DTR-TUNEL-double-positive cells to the total number of DTR-positive cells. All of the coverslips were counted blindly.

Statistical evaluation
One-way ANOVA with post hoc tests (Statview 5.01; SAS Institute, Cary, NC) determined the statistical significance of the difference between treatments. The Sheffé's test was applied as the post hoc analysis comparing data between each treatment group. A p value of <0.05 was taken as the criteria for statistical significance.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
Physiological concentrations of estrogen and androgen protect human neurons in primary culture against intracellular A_1-42-induced cell death
Human fetal brains express estrogen receptor and subtypes and androgen receptor subtype (Wilson and McPhaul, 1996; Takeyama et al., 2001). Microinjection of A_1-42 into the cytosol of neurons induces 60% cell death within 24 hr (Fig. 1A,B) (Zhang et al., 2002). Immediate incubation of the injected neurons with 2, 4, or 10 nM 17--estradiol, testosterone, and methyl testosterone significantly decreases cell death by 50% as measured by TUNEL and morphological assessments (Fig. 1A,B,D). A 1 hr preincubation with these hormones before the microinjection of A_1-42 into neurons completely protects against cell death (Fig. 1C). In contrast, the transcriptionally inactive isoform 17--estradiol, membrane-impermeable BSA-conjugated 17--estradiol, and the testosterone antagonist epitestosterone do not have any protective effects (Fig. 1A,B). These results show that physiological concentrations of estrogen and androgens (Wilson et al., 1978) protect human neurons against iA_1-42. The increased protection with preincubation indicates that the hormones alter the state of neuronal susceptibility to the iA_1-42.

View larger version (20K): [in this window] [in a new window]   Figure 1. Estrogen and androgens protect human neurons against intracellular A1-42 toxicity. A, B, TUNEL-positive cell death in human neurons in primary cultures injected with 10 nM A1-42 and incubated with 2, 4, and 10 nM 17--estradiol (17E2), 17--estradiol (17E2), BSA-17--estradiol (BSA-E2), testosterone (Test), epitestosterone (Epitest), or methyl testosterone (Methyl-test). Data represent the mean ± SEM of three independent experiments. *p < 0.002 compared with A1-42. C, TUNEL-positive cell death in human neurons preincubated with 10 nM estrogen or androgens for 1 hr before microinjections of iA1-42 and further incubated with hormones for 24 hr after the injection. Data represent the mean ± SEM of three independent experiments. *p < 0.001 compared with iA1-42 alone. D, Immunofluorescence micrographs of neurons injected with A1-42 and DTR and either left untreated (control) or treated with 2 and 4 nM 17E2 or testosterone (Test), respectively. The panels show the DTR-injected neurons stained with the DNA stain 4',6'-diamidino-2-phenylindole (DAPI) or the cell death marker TUNEL. Ctl, Control.

 
Estrogen and androgen protect against intracellular A through their respective receptors
Both estrogen and androgen receptors exist in the primary cultures of human neurons (Hammond et al., 2001; Zhang et al., 2001). However, androgens can also be aromatized into estrogen (Finkelstein et al., 1981). To determine whether each hormone is neuroprotective through its respective receptor, the effect of antagonists on hormone-mediated neuroprotection was evaluated. The estrogen receptor antagonist tamoxifen and the androgen receptor antagonist flutamide completely blocked the protection induced by estrogen and androgen, respectively (Fig. 2). Tamoxifen and flutamide treatments alone do not induce cell death in human neurons. These results show that both hormones are neuroprotective through their respective receptors.

View larger version (24K): [in this window] [in a new window]   Figure 2. Estradiol and testosterone protect against iA1-42 through their respective receptors. TUNEL-positive cell death in human neurons in primary cultures injected with A1-42 and incubated with TMX and Flut in the absence or presence of 10 nM 17--estradiol (17E2) or testosterone (Test) is shown. Data represent the mean ± SEM of three independent experiments. *p < 0.001 compared with the respective hormonal treatment. Ctl, Control.

 
Estrogen- and androgen-mediated neuroprotection against iA_1-42 requires transcriptional activity
To investigate whether the estrogen protection requires gene transcription, we first sought to identify a dominant negative form of the ER using the ERE-luciferase reporter assay in ER-positive MCF-7 cells. In the absence of 17--estradiol, there is a baseline level of estrogen receptor activity in MCF-7 cells that may be induced by trace amounts (20 pM) of estrogen in the culture serum (Fig. 3A). In the presence of 10 nM 17--estradiol for 24 hr, luciferase activity increases threefold, consistent with the level found by others in this cell line (Khan et al., 2003). The cotransfected DBD mutant ER construct abolishes estrogen-mediated gene transcription of the ERE-luciferase reporter gene and thus shows a dominant negative effect. Comicroinjection of the DBD mutant, but not the wild-type ER, with A_1-42 in human neurons also abolishes the estrogen-mediated neuroprotection against iA_1-42 (Fig. 3B). Similarly, two AR DBD mutants, 12474 and 15579, were tested as dominant negatives in androgen-responsive AR24 cells (Brooks et al., 1998). These cells were stably transfected with the AR subtype . After a 24 hr treatment with 10 nM testosterone, the AR activity increases threefold (Fig. 4A), similar to the induction levels observed with the same cDNA constructs in cultured human skin fibroblasts (Nguyen et al., 2001). The mutant 12474 decreases the androgen response by only 30-40%, whereas 15579 completely abolishes the androgen response (Fig. 5A). When injected into human neurons with A_1-42, wild-type AR but not mutant ARs decrease A toxicity in untreated or epitestosterone-treated neurons, again indicating a response to serum hormone (Fig. 4B). In neurons treated with testosterone and methyl testosterone, mutant 15579 completely inhibits and 12474 partially inhibits androgen-mediated neuroprotection against iA_1-42. Therefore, estrogen-and androgen-mediated transcription is necessary for both estrogen- and androgen-regulated neuroprotection against iA_1-42.

View larger version (23K): [in this window] [in a new window]   Figure 3. Estrogen requires transcriptional activation to protect against A1-42. A, Estrogen transcriptional activity assay using a luciferase reporter system in MCF-7 cells transfected with wild-type (WTER) or mutant (DBDER) ER and treated without (control) or with 10 nM 17--estradiol (17E2) for 24 hr. Data represent the mean ± SEM of three independent experiments. *p < 0.001 compared with control values. B, TUNEL-positive cell death in primary neurons microinjected with iA1-42 and WT-ER or DBD-ER and treated without (control) or with 17E2. Data represent the mean ± SEM of three independent experiments. *p < 0.02 compared with vector-injected cells. Ctl, Control; RLU, relative light units.

 

View larger version (28K): [in this window] [in a new window]   Figure 4. Testosterone requires transcriptional activation to protect against A1-42. A, Luciferase assay for androgen responsive element activity in AR24 cells cotransfected with the AR mutants 15579 and 12474 or empty pcDNA3 vector and treated with 10 nM testosterone for 24 hr. Data represent the mean ± SEM of three independent experiments. *p < 0.01 compared with control. B, TUNEL-positive cell death in neurons comicroinjected with A1-42 and wild-type AR (AR), 12474 AR, or 15279 AR and treated with 10 nM testosterone, methyl testosterone, or epitestosterone. *p < 0.001 compared with DTR-microinjected cells. Ctl, Control.

 

View larger version (29K): [in this window] [in a new window]   Figure 5. Hsp70 is increased in estrogen- and testosterone-treated neurons and protects against iA1-42. A, Western blot analysis of Hsp70 and-actin in 30 µg protein extracts from estrogen- or testosterone-treated neurons. B, TUNEL-positive neuronal cell death in neurons comicroinjected with iA1-42 and recombinant Hsp70 or control BSA protein compared with testosterone treatment. Ctl, Control.

 
Androgen and estrogen increase Hsp70 in human neurons, and Hsp70 is sufficient to inhibit iA_1-42-mediated neurotoxicity
Mass spectrometric analysis of proteins from neurons incubated with testosterone identified Hsp70 with an expectation value of 4 x 10^-9. Because Hsp70 has been found to interact with both A_1-42 (Fonte et al., 2002) and p53 (King et al., 2001), which is activated by iA_1-42 in neurons (Zhang et al., 2002), we pursued the potential role of Hsp70 in hormone-mediated neuroprotection. Western blot analyses confirm the increased levels of Hsp70 in estrogen- and androgen-treated neurons (Fig. 5A). Microinjection of recombinant human Hsp70 with iA_1-42 into primary neurons abolishes iA_1-42-mediated neurotoxicity to the same extent as with testosterone and estrogen treatments (Fig. 5B). We conclude from these experiments that androgen- and estrogen-mediated increases in Hsp70 cellular levels are sufficient to modulate estrogen- and androgen-mediated protection against iA_1-42.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

 
In this study, we show that: (1) physiological concentrations of both estrogen and androgen completely protect human primary neurons against iA_1-42 toxicity, (2) estrogen and androgens are neuroprotective through their respective receptors, (3) estrogen-and androgen-mediated protection against iA_1-42 depends on transcriptional activation, and (4) Hsp70, which is increased in estrogen- and testosterone-treated neurons, completely protects against iA_1-42-mediated toxicity.

The neuroprotective role of physiological concentrations of androgens and estrogens against iA_1-42 neurotoxicity is an important finding, because iA_1-42 accumulation in AD neurons precedes other pathological hallmarks and is an early event that likely leads to neuronal dysfunction and cell death (Gouras et al., 2000; Takahashi et al., 2002; Zhang et al., 2002). Except for inhibitors of - or -secretases to prevent the production of amyloid, most efforts to inhibit or remove amyloid toxicity, including vaccines, protease treatments, and anti-fibril agents, are directed at the extracellular amyloid but not intracellular amyloid toxicity. Our results indicate that sex steroids could play an important role in the early treatment of AD by preventing potential intracellular amyloid toxicity. There is presently much controversial evidence on the use of sex steroids against neurodegeneration. However, the strong neuroprotective role of these hormones shown in this study justifies additional investigations on their potential use in neurodegenerative diseases. Our results indicate that potential problems incurred in clinical trials may be avoided. First, the use of physiological levels of hormones would likely be sufficient for the protective action and may avoid undue complications caused by pharmacological doses of the hormones. Second, because both estrogens and androgens protect equally well through their respective receptors, both men and women can be treated with lower side effects. Third, understanding the underlying molecular mechanism of the action of these hormones may help target a pathway that is involved in neuroprotection against iA_1-42 toxicity while avoiding the multiple potentially detrimental actions of these hormones.

Increased levels of Hsp70 are not unique to estrogen- and androgen-treated neurons. Several studies have found increased expression of Hsp70 in various hormone-treated cell types (Tang et al., 1995; Jones et al., 2000; Lu et al., 2002; Gehring, 2004). The fact that Hsp70 can completely prevent iA_1-42-mediated toxicity indicates only that Hsp70 is sufficient for neuroprotection against iA_1-42 toxicity but does not rule out the possibility that other effects of the steroid hormones on neurons could also be neuroprotective. However, our results corroborate those showing that Hsp70 can protect against polyglutamine toxicity (Warrick et al., 1998; Jana et al., 2000; Cummings et al., 2001), -synuclein toxicity (Auluck et al., 2002), and iA_1-42 toxicity (Fonte et al., 2002; Magrane et al., 2004) in flies, cell cultures, and mice, respectively. Most importantly, prevention by Hsp70 of a progressive paralysis phenotype caused by overexpression of iA_1-42 in muscle cells of Caenorhabditis elegans indicates a functional protection against iA_1-42 (Fonte et al., 2002).

The molecular mechanism underlying Hsp70 neuroprotection against neurodegenerative conditions is not clear. In our system, we have demonstrated previously that iA_1-42 induces human neuronal apoptosis through the activation of p53 and Bax (Zhang et al., 2002). Hsp70 could sequester p53 in the cytosol and prevent its translocation to the nucleus and activation of apoptosis (King et al., 2001; Zylicz et al., 2001). An alternative possibility is that Hsp70 interacts directly with iA_1-42. Fonte et al. (2002) have shown interaction between iA_1-42 and Hsp70 in C. elegans that is consistent with the ability of Hsp70 to bind peptides and denatured proteins. Finally, Hsp70 has been implicated recently in steroid-mediated transcriptional activation by forming a complex with Bag-1 and steroids (Gehring, 2004). Hsp70 may enhance steroid-mediated transcriptional activation of prosurvival genes. These are issues that will be difficult to resolve in human neurons considering the natural predisposition of A_1-42 to form aggregates that can interact nonspecifically with proteins and the resistance of human neurons in culture to infections or transfections, thereby limiting our studies to single-cell analyses (our unpublished observations).

In summary, we have shown that physiological concentrations of estrogen and androgens protect human neurons from iA_1-42-mediated toxicity and increase Hsp70 in these neurons. Hsp70 completely protects against iA_1-42-mediated toxicity. This study therefore identifies in Hsp70 a common downstream target of estrogen and androgen that is involved in neuroprotection.

	Footnotes

 
Received March 12, 2004; revised April 21, 2004; accepted April 22, 2004.

This work was funded by the Canadian Institute for Health Research, the National Institutes of Health, the Fond de Rechercheen Santé du Québec (A.L.), and the Alzheimer Society of Canada (Y.Z.).We are grateful for the technical support of Jennifer Hammond pertaining to cell cultures. We thank Dr. Sylvie Mader for the ER wild-type and mutant constructs.

Correspondence should be addressed to Dr. Andréa LeBlanc, The Bloomfield Center for Research in Aging, Lady Davis Institute for Medical Research, The Sir Mortimer B. Davis Jewish General Hospital, 3755 Chemin Côte Ste-Catherine, Montréal, Québec, Canada, H3T 1E2. E-mail:andrea.leblanc{at}mcgill.ca.

Copyright © 2004 Society for Neuroscience 0270-6474/04/245315-07$15.00/0

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