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. 2004 Jul 28;24(30):6799–6809. doi: 10.1523/JNEUROSCI.5463-03.2004

β-Amyloid Peptide at Sublethal Concentrations Downregulates Brain-Derived Neurotrophic Factor Functions in Cultured Cortical Neurons

Liqi Tong 1, Robert Balazs 1, Phillip L Thornton 1, Carl W Cotman 1
PMCID: PMC6729714  PMID: 15282285

Abstract

The accumulation of β-amyloid (Aβ) is one of the etiological factors in Alzheimer's disease (AD). It has been assumed that the underlying mechanism involves a critical role of Aβ-induced neurodegeneration. However, low levels of Aβ, such as will accumulate during the course of the disease, may interfere with neuronal function via mechanisms other than those involving neurodegeneration. We have been testing, therefore, the hypothesis that Aβ at levels insufficient to cause degeneration (sublethal) may interfere with critical signal transduction processes. In cultured cortical neurons Aβ at sublethal concentrations interferes with the brain-derived neurotrophic factor (BDNF)-induced activation of the Ras-mitogen-activated protein kinase/extracellular signal-regulated protein kinase (ERK) and phosphatidylinositol 3-kinase (PI3-K)/Akt pathways. The effect of sublethal Aβ1-42 on BDNF signaling results in the suppression of the activation of critical transcription factor cAMP response element-binding protein and Elk-1 and cAMP response element-mediated and serum response element-mediated transcription. The site of interference with the Ras/ERK and PI3-K/Akt signaling is downstream of the TrkB receptor and involves docking proteins insulin receptor substrate-1 and Shc, which convey receptor activation to the downstream effectors. The functional consequences of Aβ interference with signaling are robust, causing increased vulnerability of neurons, abrogating BDNF protection against DNA damage- and trophic deprivation-induced apoptosis. These new findings suggest that Aβ engenders a dysfunctional encoding state in neurons and may initiate and/or contribute to cognitive deficit at an early stage of AD before or along with neuronal degeneration.

Keywords: β-amyloid, BDNF, CREB, MAPK, cortical neurons, PI3-K

Introduction

Alzheimer's disease (AD) is characterized by a progressive decline in cognitive functions. Hallmarks of the neuropathology include the accumulation of tangles, amyloid-β (Aβ)-containing plaques, dystrophic neurites, and loss of synapses and neurons (Selkoe, 1999). It generally is believed that Aβ peptides contribute significantly to the pathogenesis of the disease, although the mechanisms are not understood clearly. Transgenic animals overexpressing AD-associated mutant β-amyloid precursor protein (APP) mimic certain features of AD, including the deposition of amyloid plaques and the development of cognitive deficits. However, although neurite degeneration is observed, neuron loss is not a consistent feature of the phenotype (Hsiao et al., 1996; Chapman et al., 1999; Hsia et al., 1999; Hardy and Selkoe, 2002). Furthermore, in certain animal models impaired performance in behavioral tests precedes abundant amyloid plaque deposition (Holcomb et al., 1998), suggesting that nondegenerative mechanisms may contribute to cognitive decline. Similarly, studies on postmortem brains are consistent with the view that cognitive decline may precede the formation of plaques and neurodegenerative changes (Morris et al., 1996; Lue et al., 1999; Naslund et al., 2000; Snowdon et al., 2000). Thus, although it is well documented that Aβ peptides can cause neurodegeneration both in vivo and in vitro (Yankner, 1996), it seems that impairment of neuronal plasticity, including cognition, may precede both high levels of Aβ accumulation and neuron loss in the brain.

AD is a progressive disease, and Aβ may be present in the brain at sublethal concentrations for extended periods before the overt manifestation of the disorder. Recently, we proposed that Aβ at levels not compromising survival may affect neuronal function via critical signal transduction processes that mediate plastic changes, including those involved in learning and memory (Tong et al., 2001). In that study we observed that sublethal Aβ1-42 interferes with neuronal activity-dependent signaling, suppressing activation of the transcription factor cAMP response element-binding protein (CREB) that plays a critical role in learning and memory in different species (Bourtchuladze et al., 1994; Tully, 1997) and also has cell survival-promoting effects (Bonni et al., 1999).

One of the CREB target genes is brain-derived neurotrophic factor (BDNF), and the Aβ1-42 treatment interfered with the CREB activation-induced transcription of the BDNF gene (Tong et al., 2001). BDNF has an important role, in its own right, in promoting neuronal survival, differentiation, and synaptic plasticity (Thoenen, 2000; Huang and Reichardt, 2001). In the present study we examined, therefore, the influence of sublethal concentrations of Aβ1-42 on BDNF-induced signaling and neuroprotection in cultured rat cortical neurons, because BDNF might be not only a target but also one of the effectors of Aβ1-42 action. The effects of BDNF are mediated by TrkB receptor-induced activation of key signaling pathways, including phospholipase Cγ (PLCγ), Ras-mitogen-activated protein kinase/extracellular signal-regulated protein kinase (MAPK/ERK), and phosphatidylinositol 3-kinase (PI3-K)/Akt pathways, leading to the activation of critical transcription factors such as CREB and Elk-1, which play crucial roles in neuronal physiology, including synaptic plasticity (Finkbeiner et al., 1997; Tully, 1997; Wasylyk et al., 1998; Huang and Reichardt, 2001).

Our current observations show that Aβ1-42 at sublethal levels suppresses BDNF-induced activation of selective signaling pathways by interfering at the level of docking proteins that mediate signaling to Ras-MAPK/ERK and PI3-K/Akt pathways. Taken together, our observations support a model in which sublethal Aβ interferes with signaling critical for neuronal function and plasticity and thus may contribute to the cognitive impairment that precedes the development of the AD characteristic neuropathology.

Materials and Methods

Cell culture. Cultures greatly enriched in cortical neurons from embryonic day 18 rat fetuses were prepared as described previously (Pike et al., 1993). Cells plated at 2.5 × 104 cells/cm2 were cultured in poly-l-lysine-treated multiwell plates and maintained in serum-free optimal DMEM supplemented with B27 components (Invitrogen, Carlsbad, CA). When cells were exposed to Aβ, the medium was switched to DMEM/B27 containing Aβ. Cultures were maintained for 5 d before treatments. Neuronal survival was determined at 5 d in vitro (5 DIV) by trypan blue exclusion (Pike et al., 1993) or by use of the MTT assay (Ivins et al., 1999). Early apoptotic changes were assessed by using the Annexin V FLUOS staining kit (Roche Biochemicals, Indianapolis, IN).

Cells were treated with tetrodotoxin (TTX; 1 μm) and amino-5-phosphonovaleric acid (100 μm) 2 hr and 30 min, respectively, before exposure to Aβ to reduce endogenous synaptic activity and to block glutamate release induced by BDNF (Li et al., 1998; Numakawa et al., 2001) to reduce the basal level of activated signaling molecules (Chandler et al., 2001). Cells were treated with Aβ for 2 hr before the addition of BDNF (PeproTech, Rocky Hill, NJ). After 10-15 min of incubation with BDNF the cells were lysed and the preparations subjected to either electrophoresis or immunoprecipitation.

Aβ peptides [Aβ1-42 and Aβ1-42(R) with random amino acid sequence] were synthesized by solid-phase Fmoc [N-(9-fluorenyl) methoxycarboxyl] amino acid chemistry, purified by reverse-phase HPLC, and characterized by electrospray mass spectrometry as previously described (Burdick et al., 1992; Pike et al., 1993). A stock solution of Aβ (1 mm) was prepared in distilled water and used after one freeze-thaw cycle. Preparations of Aβ1-42 oligomers were obtained from the same lot of Aβ1-42 peptides as the β-sheet containing Aβ1-42 preparations described above to facilitate the comparison of the two preparations. Solutions of Aβ1-42 oligomers were prepared as previously described (Oda et al., 1995; Lambert et al., 1998). In brief, Aβ1-42 (100 μm) in cold DMEM was vortexed and incubated at 4-8°C for 24 hr. Solutions were centrifuged at 14,000 × g for 10 min to remove large aggregates, and the supernatant was used for all assays. In agreement with the published reports, microscopic examination of these preparations indicated that the supernatant contained no large aggregates.

Test for phosphatidyl serine externalization (annexin staining). Cells were grown on glass coverslips as above. At 5 DIV the cultures received Aβ1-42, and after 2 hr the medium was removed and replaced with DMEM/B27. After an additional 2 hr period annexin V-FLUOS and propidium iodide were added, and the cultures were viewed with confocal microscopy after 30 min of staining.

Western blots. Cultures of cortical neurons were lysed in SDS-sample buffer, and proteins, resolved by 10% SDS-PAGE, were transferred to polyvinylidene difluoride membrane. Membranes were incubated in Tris-buffered saline (TBS) containing 0.1% Tween and 5% nonfat milk for 60 min at room temperature to block nonspecific binding. Membranes were incubated additionally for 2 hr at room temperature in the presence of the following antibodies as indicated: from Upstate Cell Signaling (Charlottesville, VA), phosphorylated CREB (P-CREB; detects CREB phosphorylated at Ser133; 1:2000), total CREB (T-CREB; 1:2000), Shc (the antibody recognizes all isoforms; 1:1000), PLCγ (1:1000), total TrkB (T-TrkB; 1:1000); from Cell Signaling Technology (Beverly, MA), phosphorylated MAPK/ERK (P-MAPK; detects p44/42 MAPK phosphorylated at Thr202 and Tyr204; 1:2000), total MAPK (T-MAPK; 1:2000), phosphorylated Raf-1 (P-Raf-1; detects Raf-1 phosphorylated at Ser388; 1:1000), phosphorylated MEK1/2 (P-MEK1/2; detects MEK1/2 phosphorylated at Ser217/221; 1:1000), total MEK1/2 (T-MEK1/2; 1:1000), phosphorylated Elk-1 (P-Elk-1; detects Elk-1 phosphorylated at Ser383; 1:1000), total Elk-1 (T-Elk-1; 1:1000), phosphorylated Akt (P-Akt; detects Akt phosphorylated at Ser473; 1:1000), total Akt (T-Akt; 1:1000), phosphorylated TrkB (P-TrkB; detects TrkB phosphorylated at Tyr490; 1:500). Membranes then were treated with HRP-conjugated secondary antibodies for 1 hr, followed by four washes with TBS containing 0.1% Tween. Immunolabeling was detected by enhanced chemiluminescence (Amersham Biosciences, Piscataway, NJ) according to the recommended conditions. Immunoreactivity was quantified by using densitometric analysis.

Immunoprecipitation. Cells were lysed in 500 μl of immunoprecipitation buffer [1% Triton X-100 plus (in mm) 150 NaCl, 50 Tris, pH 8.0, 0.2 sodium orthovanadate, 0.2 phenylmethylsulfonyl fluoride, and 1 mg/ml each pepstatin, leupeptin, and antipain]. Lysates were centrifuged at 10,000 × g for 30 min, and protein concentration of the clarified lysates was determined by the Micro-BCA protein assay (Pierce, Rockford, IL). Proteins were immunoprecipitated with anti-insulin receptor substrate-1 (anti-IRS-1)-, anti-Shc-, or agarose-linked anti-phosphotyrosine antibodies at 4°C overnight. After immunoprecipitation with anti-IRS-1 or anti-Shc antibodies the samples were rotated in the presence of protein G-Sepharose at 4°C for 2 hr. The immune complexes were pelleted by centrifugation at 10,000 × g at 4°C for 1 min. The supernatant was decanted, and the pellet was washed with 1 ml of immunoprecipitation buffer. These steps were repeated three times; finally, the pellet was suspended in 60 μl of SDS-sample buffer (62.5 mm Tris, pH 6.8, 2% SDS, 10% glycerol, 5% β-mercaptoethanol, 0.01% bromphenol blue). Proteins of the suspended immunoprecipitate (30 μl) were separated on a 10% SDS-PAGE gel. The immunoprecipitates were analyzed by Western blotting with anti-phosphotyrosine 4G10 (Upstate Cell Signaling) or PLCγ (Upstate Cell Signaling) antibodies.

Immunocytochemistry. Cultures were fixed with 4% paraformaldehyde in 0.1 m PBS, pH 7.4. After fixation the cultures were treated with a solution of 3% aqueous H2O2 for 3 min and then briefly rinsed with PBS. Cultures next were incubated with PBS containing 5% bovine serum albumin (BSA) and 0.3% Triton X-100 at room temperature for 1 hr, followed by additional incubation at 4°C in PBS/5% BSA containing the rabbit polyclonal IgG against P-CREB (1:2000; Upstate Biotechnology, Lake Placid, NY). Cultures then were rinsed in buffer and incubated in biotinylated goat anti-rabbit IgG. After a buffer rinse the cultures were incubated in the presence of avidin-biotin complex (Vector Laboratories, Burlingame, CA) for 90 min. They were rinsed in 0.1 m Tris-HCl, pH 7.6, and treated with diaminobenzidine tetrahydrochloride (0.05% in Tris-HCl) and 0.01% hydrogen peroxide for 5-10 min. Reactions were stopped by rinsing the cultures with PBS.

Cortical neuron transfection and luciferase assay. Cortical neurons were transfected with the plasmid pCRE-Luc containing the cAMP response element (CRE) sequence (TGACGTCA) and pSRE-Luc containing the serum response element (SRE) sequence (CCATATTAGG) (Stratagene, La Jolla, CA) at 3 DIV with a procedure described by Myers et al. (1998). Briefly, cultures in six-well 35 mm dishes were transfected in the presence of Lipofectamine 2000 (Invitrogen) according to the manufacturer's instructions. Each well was transfected with 1 μg of reporter plasmid and 0.1 μg of pRL-CMV (Promega, Madison, WI), a CMV-luciferase control plasmid to normalize CRE and SRE activity. At 40 hr after transfection the cultures received 50 ng/ml BDNF for 9 hr; then the plates were washed twice with cold PBS, and the cells were lysed with 200 μl of lysis buffer (Promega). Cell extract (20 μl) was used for a dual-luciferase reporter assay (Promega) according to the manufacturer's instructions.

Akt activity assay. Akt activity was determined with an Akt assay kit (Cell Signaling Technology) according to the manufacturer's instruction. The phosphorylation of a substrate of Akt (glycogen synthase kinase, GSK-3α/β) was measured by using immunoprecipitated Akt from cell lysates. Cell extracts (200 μl) were incubated for 2 hr with immobilized Akt 1G1 monoclonal antibody. After extensive washing the kinase reaction was performed in the presence of 200 μm cold ATP and GSK-3α/β substrate. Phosphorylation of GSK-3α/β was measured by Western blots, using phospho-GSK-3α/β antibody (detects GSK-3α containing phosphorylated Ser21 and GSK-3β containing Ser9).

Deprivation from trophic support. It was established that BDNF can protect neurons from cell death induced by serum deprivation (Hetman et al., 1999). Our cultures were maintained in the B27 serum-free medium that contains a great number of trophic ingredients providing comparable support for neuron survival as serum does but that prevents the proliferation of glial cells. We observed that deprivation from B27, like that from serum, compromised neuronal survival, thus permitting the testing of the effect of BDNF and Aβ1-42 on the survival of the deprived cells. In these studies the B27-containing medium was removed from the cultures at 4-6 DIV. Cells were washed twice with DMEM and then incubated in DMEM for 36 hr in the absence or presence of 10 ng/ml BDNF ± 5 μm1-42. Control cells were treated the same way but were incubated in B27-containing DMEM.

Camptothecin treatment. At 4-6 DIV the cortical neurons were treated with 5 μm camptothecin for 24 hr, after a 1 hr pretreatment with 10 ng/ml BDNF or vehicle in the presence or absence of 5 μm1-42. Neuronal survival was determined by trypan blue exclusion.

Results

In a previous study, we observed that Aβ1-42 at sublethal concentrations inhibits neuronal activity-dependent phosphorylation of CREB and CREB-mediated gene expression, as exemplified by the suppression of the transcription of the CREB target BDNF gene (Tong et al., 2001). BDNF, a member of neurotrophin family, is an important factor for both the developing and mature neurons and has a pleiotropic influence on nerve cells, including effects on synaptic transmission and neuronal plasticity, in addition to regulating the survival, differentiation, and maintenance of specific neuronal populations (for review, see Thoenen, 2000; Huang and Reichardt, 2001). Mice deficient in either BDNF or its receptor TrkB exhibit impaired dendritic and axonal arborization, synaptic activity, and neuronal plasticity, including impairment in long-term potentiation (LTP) and learning and memory processes (Korte et al., 1995; Patterson et al., 1996; Causing et al., 1997; Martinez et al., 1998; Minichiello et al., 1999). In the current study we examined whether Aβ1-42, which at sublethal levels interferes with BDNF production, has an influence on BDNF-induced signal transduction, including CREB activation.

1-42 at the concentration range of 1-10 μm did not compromise cell survival assessed by the technique of either trypan blue exclusion (Fig. 1) or MTT reduction (data not shown). Under our experimental conditions the toxic effect is manifested after exposure to ≥20 μm of Aβ1-42 for 24 hr (Ivins et al., 1999). Although neurons remained viable in the presence of 1-10 μm1-42 during the experimental period that was studied, these sublethal concentrations may have triggered early apoptotic processes. Probing for such early changes, we demonstrated previously that activation of caspases, which play an important role in Aβ1-42-induced apoptosis, is not involved in the sublethal Aβ1-42-induced suppression of the neuronal activity-evoked increase in phosphorylated CREB levels (Tong et al., 2001). As an early marker of apoptosis, here we examined the externalization of phosphatidyl serine (PS) to the outer leaflet of the plasma membrane, using annexin IV binding for detection (Martin et al., 1995). We estimated this early marker of apoptosis after a 4 hr exposure to 1-10 μm1-42, which is longer than the 2 hr Aβ treatment that was the routine in most of the current experiments, and we observed no indication of PS externalization (data not shown).

Figure 1.

Figure 1.

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Viability of cortical neurons after Aβ1-42 treatment. Cortical neuronal cultures at 5 DIV were treated with Aβ1-42 at the indicated concentrations and length of time. Viability was determined by the trypan blue exclusion assay. Data shown are the mean ± SE (n = 4). In three separate experiments cell viability was measured with the MTT assay, which showed no significant reduction after exposure to 10 μm1-42 for 24 hr.

BDNF-induced activation of CREB is suppressed by sublethal concentrations of Aβ1-42

We confirmed previous observations [Iida et al. (2001) and references therein] and found that BDNF elicited a marked increase in cultured cortical neurons in the level of CREB phosphorylated at the critical Ser133 (P-CREB) (Fig. 2). Pretreatment with Aβ1-42 in the subtoxic range for 2 hr resulted in a concentration-dependent decrease in the effect of BDNF on P-CREB levels without affecting the total amount of CREB (T-CREB) (Fig. 2A,B). The effect was specific, because Aβ1-42 with random sequence of amino acid residues [Aβ(R)] failed to influence BDNF-induced activation of CREB (Fig. 2C). Furthermore, 2 hr exposure to Aβ1-42 alone had no significant effect on basal P-CREB levels (Fig. 2E). We also examined the effect of Aβ1-42 treatment on BDNF-induced CREB activation via immunocytochemistry (Fig. 2D). BDNF elicited a pronounced increase in P-CREB immunoreactivity in almost all neurons, and this effect was attenuated markedly by exposure to 5 μm1-42.

Figure 2.

Figure 2.

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Pretreatment with sublethal concentrations of Aβ1-42 (5 or 10 μm) for 2 hr decreased the elevation of phosphorylated CREB levels induced by BDNF (50 ng/ml, 10 min). A, Western blot analysis of CREB phosphorylated at Ser133 (P-CREB) and total CREB (T-CREB). Aβ1-42 treatment resulted in a concentration-dependent decrease in the level of P-CREB but, considering all experiments (n = 3), had no significant effect on T-CREB levels. B, Quantification of the effect of pretreatment with 1, 5, or 10 μm1-42 (A1, A5, A10; A, here and in all other figures, stands for Aβ1-42). Estimates are the mean ± SEM (n = 3) expressed in terms of P-CREB levels obtained in the BDNF-exposed cultures (B, here and in all other figures, stands for BDNF). The effect of Aβ1-42 was significant (*p < 0.05, unpaired Student's t test). C, Pretreatment with 10 μm1-42 with random amino acid sequence [Aβ(R)] had no significant influence on the BDNF-induced increase of P-CREB levels. D, Immunohistochemical analysis of P-CREB. P-CREB immunoreactivity increased in BDNF-stimulated cultures (b) compared with unstimulated control (a). BDNF-induced increase in P-CREB immunoreactivity was suppressed by Aβ1-42 (5 μm) treatment (c). E, Exposure of the cultures to Aβ1-42 for 2 hr had no effect on P-CREB levels. In three experiments P-CREB levels in the presence of 5 and 10 μm1-42, respectively, were 104 ± 2 and 105 ± 6% of basal. F, Analysis of CRE-mediated transcriptional activity. Cortical neurons at 3 DIV were transfected with plasmid pCRE-Luc containing CRE sequences and a luciferase reporter gene (see Materials and Methods). Cells transfected with a CMV-luciferase control plasmid served to normalize CRE activity. After 40 hr the cultures were switched to fresh medium and incubated for 1 hr in the presence or the absence of 5 μm1-42. Transfected cortical cultures were incubated for an additional 9 hr either with or without the addition of 50 ng/ml BDNF, and transcriptional activity was measured by the luciferase assay. Aβ1-42 treatment decreased the BDNF-induced transcriptional activity of CRE. Estimates are the mean ± SEM (n = 3) expressed in terms of BDNF-induced transcriptional activity. The effect of Aβ1-42 was significant (*p < 0.05, unpaired Student's t test).

To examine the consequences of the suppression of Aβ at sublethal concentrations on BDNF-mediated CREB activation, we analyzed the effect of the peptide on transcriptional activity of a promoter construct containing CRE sequences. Effects were monitored by a transient transcription activity assay with luciferase as a reporter gene. BDNF increased the CRE transcription activity, and pretreatment with Aβ1-42 reduced by ∼50% the induction by BDNF (Fig. 2F).

Effect of sublethal concentrations of Aβ1-42 on MAPK activation

Various pathways can mediate CREB activation. In our previous study CREB phosphorylation was evoked by the stimulation of neurons with NMDA (10 μm) or elevated K+ (30 mm), and under these conditions pathways other than the Ras/MAPK pathway are involved primarily in CREB activation (Iida et al., 2001). In the present work the neurons were exposed to BDNF, when the activation of the Ras-MAPK pathway plays a dominant role in CREB phosphorylation (Iida et al., 2001).

MAPKs are highly expressed in neurons, and it has been shown that the ERK isoforms, in particular, are important regulators of synaptic plasticity (Sweatt, 2001) in addition to their more general critical role in cell proliferation and differentiation (Marshall, 1994). Because BDNF-induced CREB activation was compromised by the Aβ1-42 treatment and the MAPK/ERK pathway seems to play a dominant role in BDNF signaling to CREB, we examined the influence of sublethal level of Aβ1-42 on the BDNF-induced activation of MAPK (Fig. 3A,B).

Figure 3.

Figure 3.

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Pretreatment with sublethal Aβ1-42 (5 or 10 μm) decreased the BDNF-induced increase in the level of phosphorylated p42- and p44-MAPK/ERK elicited by stimulation with BDNF (50 ng/ml, 10 min). A, Western blot analysis showed that Aβ1-42 exposure resulted in a concentration-dependent decrease in the level of phosphorylated p42- and p44-MAPK (p42- and p44-P-MAPK). B, Quantification of the effects of pretreatment with 5 or 10 μm1-42. Estimates are the mean ± SEM (n = 3) expressed in terms of p42- and p44-P-MAPK levels obtained in the BDNF-exposed cultures. Effects of 5 and 10 μm1-42 (A5, A10) were significant (*p < 0.05, unpaired Student's t test).

Under our experimental conditions, which included transmission blockade via TTX and the inhibition of NMDA receptors, the basal level of dual-phosphorylated MAPK/ERK was very low (Chandler et al., 2001). Exposure to BDNF (50 ng/ml) for 10 min caused a robust increase in the amount of both the phosphorylated p42 and p44 isoforms of MAPK. Pretreatment with sublethal concentrations of Aβ1-42 for 2 hr had no significant effect on the basal level of phosphorylated MAPK (data not shown) but resulted in a decrease in the BDNF-elicited activation of both MAPK isoforms (Fig. 3A,B).

Diffusible Aβ1-42 oligomers decrease with high-potency BDNF-induced signal transduction

There is evidence that diffusible Aβ oligomers are more potent than the conventional fibrillar Aβ preparations in compromising neuronal function and survival (Lambert et al., 1998; Walsh et al., 2002). We also observed previously that, in comparison with our conventional Aβ1-42 preparation, the diffusible oligomeric form of Aβ1-42 (see Materials and Methods) is more potent both in inducing neurotoxicity and at sublethal concentrations interfering with high K+-induced CREB phosphorylation (Tong et al., 2001). Here we examined the effect of this Aβ1-42 oligomer preparation on the BDNF-induced activation of the CREB. We confirmed our earlier observation that the Aβ1-42 oligomers are neurotoxic at concentrations ≥1 μm (data not shown). At the sublethal concentration of 200 nm the Aβ1-42 oligomers suppressed the BDNF-induced increase in the amount of the phosphorylated CREB (Fig. 4A,B).

Figure 4.

Figure 4.

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A preparation comprising diffusible Aβ1-42 oligomers interferes with high potency with BDNF-induced signaling. A, Western blots showing that pretreatment (1 hr) with an Aβ1-42 oligomer preparation at the sublethal concentration of 200 nm compromised the increase in P-CREB levels induced by BDNF (50 ng/ml, 10 min). B, Quantification of the effect of 200nm1-42 oligomers. Estimates are the mean ± SEM (n = 3) expressed in terms of P-CREB levels obtained in BDNF-treated cultures. The effect of 200 nm1-42 oligomers was significant (*p < 0.05, unpaired Student's t test). C, Western blot analysis of P-MAPK. Pretreatment with 200 nm1-42 oligomers for 1 hr attenuated the increase in P-MAPK levels by exposure to 50 ng/ml BDNF for 10 min. D, Quantification of the effect of pretreatment with 200 nm1-42 oligomers for 1 hr. Estimates are expressed in terms of P-MAPK levels obtained in the BDNF-treated cultures; they are the mean ± SEM from three independent experiments. The effect of Aβ1-42 oligomers was significant (*p < 0.05, unpaired Student's t test).

We also examined the effect of a sublethal concentration of the Aβ1-42 oligomer preparation on the BDNF-induced activation of the MAPK. Pretreatment with 200 nm1-42 oligomers decreased significantly the BDNF-induced increase in the amount of the phosphorylated p42 and p44 isoforms of MAPK (Fig. 4C,D).

Effect of sublethal concentrations of Aβ1-42 on the activation of Elk-1, a transcription factor downstream of MAPK/ERK

ERK activated as a result of BDNF-induced signal transduction can translocate to the nucleus and phosphorylate transcription factors, including Elk-1. Elk-1 is a member of the ternary complex factor (TCF) family (Wasylyk et al., 1998) and functions as a nuclear transcriptional activator via its association with serum response factor (SRF) in a ternary complex on the SRE sequence that is present in the promoter of many genes, including immediate early genes (Wasylyk et al., 1998). Exposing cortical neurons to BDNF increased the level of phosphorylated Elk-1 (P-Elk-1) (Fig. 5A). Pretreatment with 5 or 10 μm1-42 caused a marked decrease in the amount of P-Elk-1 in the BDNF-treated cultures (Fig. 5A,B).

Figure 5.

Figure 5.

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Pretreatment with Aβ1-42 at sublethal concentrations decreased the level of BDNF-activated transcription factor Elk-1 (P-Elk-1) and the transcriptional activity of a serum response element-containing (SRE) construct. A, The phosphorylation of Elk-1 was examined by the use of an antibody against phosphorylated Elk-1 (P-Elk). Pretreatment with 5 or 10 μm1-42 for 2 hr attenuated the BDNF-induced increase in P-Elk-1 but had no significant effect on the total amount of Elk-1 (T-Elk). B, Quantification of the effects of pretreatment with 5 or 10 μm1-42 (B + A5 or B + A10). Estimates are the mean ± SEM (n = 3) expressed in terms of P-Elk-1 levels induced by BDNF (B). Effects of 5 and 10 μm1-42 (A5, A10) were significant (*p < 0.05, unpaired Student's t test). C, Analysis of SRE-mediated transcriptional activity. Cortical neurons at 3 DIV were transfected with plasmid pSRE-Luc containing SRE sequences and a luciferase reporter gene (see Materials and Methods). Cells transfected with a CMV-luciferase plasmid served to normalize SRE activity. After 40 hr the cultures were switched to fresh medium and incubated for 1 hr in the presence or the absence of 5 μm1-42. Transfected cortical cultures were incubated for an additional 9 hr either with or without the addition of 50 ng/ml BDNF, and transcriptional activity was measured by the luciferase assay. Aβ1-42 treatment decreased the BDNF-induced transcriptional activity of SRE. Estimates are the mean ± SEM (n = 3) expressed in terms of BDNF-induced transcriptional activity. The effect of Aβ1-42 was significant (*p < 0.05, unpaired Student's t test).

To evaluate the consequences of the action of sublethal concentrations of Aβ on Elk-1 mediated gene expression, we analyzed the effect of the peptide on transcriptional activity of promoter constructs containing SRE sequences. The effects were monitored with a transient transcription activity assay with luciferase as a reporter gene. BDNF increased the SRE transcription activity, and pretreatment with Aβ1-42 reduced the induction by BDNF by ∼50% (Fig. 5C).

Sublethal concentrations of Aβ1-42 suppressed BDNF-induced signal transduction upstream of MAPK

Next we examined whether the interference by Aβ1-42 with the BDNF-induced activation of MAPK/ERK is attributable to effects at steps in the signaling cascade upstream of MAPK. MAPK is activated by MEK (MAPK kinase or MAPKK) that is, in turn, phosphorylated by activated c-Raf (Marshall, 1994). The levels of phosphorylated Raf-1 (P-Raf-1) and phosphorylated MEK (P-MEK1/2) in cortical neurons were examined by Western blotting with antibodies specific to P-Raf-1 and phosphorylated MEK1/2, respectively. BDNF exposure elicited an increase in the levels of both the P-Raf (Fig. 6A,B) and P-MEK1/2 (Fig. 6C,D). Pretreatment with 5 μm1-42 for 2 hr resulted in a significant suppression of the BDNF-induced increase in activated Raf-1 and MEK1/2 content without influencing the total amount of Raf-1 (T-Raf-1) and MEK1/2 (T-MEK1/2).

Figure 6.

Figure 6.

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Sublethal Aβ1-42 treatment decreased the phosphorylated levels of protein kinases in the MAPK cascade (P-Raf and P-MEK). A, The phosphorylation of Raf was examined by the use of an antibody against phosphorylated Raf-1 (P-Raf). Pretreatment with 5 μm1-42 for 2 hr attenuated the BDNF-induced increase in P-Raf. B, Quantification of the effects of pretreatment with 5 μm1-42. Estimates are the mean ± SEM (n = 3) expressed in terms of P-Raf levels induced by BDNF (represented by B). Effects of 5 μm1-42 (B + A) were significant (*p < 0.05, unpaired Student's t test). C, Pretreatment with 5 μm1-42 decreased the BDNF-induced elevation in the level of phosphorylated MEK1/2 (P-MEK1/2). D, Quantification of the effects of pretreatment with 5 μm1-42 on BDNF-induced MEK1/2 phosphorylation. Estimates are the mean ± SEM (n = 3) expressed in terms of P-MEK1/2 levels induced by BDNF. Effects of 5 μm1-42 (B + A) were significant (*p < 0.05, unpaired Student's t test).

Sublethal levels of Aβ1-42 and the BDNF-induced activation of the PI3-K pathway

BDNF activates, in addition to the Ras-MAPK pathway, signaling via PI3-K (Huang and Reichardt, 2001). PI3-K generates 3′-phosphorylated phosphoinositides that act via multiple mechanisms to regulate the downstream effectors of PI3-K, including protein kinase B or Akt (Datta et al., 1999). The increase in 3′-phosphorylated phosphoinositides results in the translocation of Akt from cytoplasm to the inner surface of plasma membrane. A conformational change after lipid binding permits the activation of Akt via phosphorylation of Thr308 and Ser473 by a protein kinase complex containing 3′-phospholipid-dependent protein kinases (PDK). Activated Akt is a major factor mediating the cell survival-promoting effect of neurotrophins (Bonni et al., 1999), including the effect of BDNF in preventing cell death induced by serum deprivation (Hetman et al., 1999). To investigate the effect of Aβ1-42 on the activation of the PI3-K/Akt pathway, we examined the level of Akt phosphorylated at the critical Ser473 residue, using a specific antibody in Western blotting. Exposure of cortical neurons to BDNF resulted in a marked increase in the level of activated Akt (Fig. 7). Pretreatment with Aβ1-42 suppressed this response in a concentration-dependent manner (Fig. 7A,B). We also examined the effect of Aβ1-42 on Akt activity, which was determined by estimating the phosphorylation of an Akt substrate, GSK-3α/β, using immunoprecipitates obtained from cell lysates treated with Akt-specific antibodies. BDNF induced a massive >10-fold increase in Akt kinase activity (Fig. 7C). Aβ1-42 alone failed to affect the basal level of activated CREB (Fig. 2E) or MAPK/ERK (data not shown) but elicited a slight increase (50 ± 13% above basal level) in Akt activity that was similar to the effect of the peptide on PC12 and SH-SY5Y neuroblastoma cells (Martin et al., 2001; Wei et al., 2002). The effect of Aβ1-42 pretreatment on the robust increase in the BDNF-evoked Akt activity was, however, a suppression by >50% (Fig. 7C,D).

Figure 7.

Figure 7.

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1-42 treatment decreased BDNF-induced Akt activation. A, Phosphorylated Akt (P-Akt) levels were determined with an antibody specific to P-Akt. Exposure to BDNF (50 ng/ml) for 10 min increased the amount of P-Akt. Pretreatment with 5 or 10 μm1-42 suppressed the effect of BDNF. Aβ1-42 had no effect on total Akt (T-Akt) levels. B, Quantification of the effect of pretreatment with 5 or 10 μm1-42. Estimates are the mean ± SEM (n = 3) expressed in terms of P-Akt levels obtained in the BDNF-exposed cultures. The effect of Aβ1-42 at 10 μm was significant (*p < 0.05, unpaired Student's t test). C, Pretreatment with 10 μm1-42 decreased BDNF-induced Akt activity, measured by the phosphorylation of glycogen synthase kinase-3α/β (GSK-3α/β), a substrate of Akt, using immunoprecipitated Akt from cell lysates as described in Materials and Methods. D, Quantification of the effects of pretreatment with 10 μm1-42. Estimates are the mean ± SEM (n = 3) expressed in terms of phosphorylated GSK-3α/β levels obtained in the BDNF-exposed cultures. The effect of Aβ1-42 was significant (*p < 0.05, unpaired Student's t test).

Effect of Aβ1-42 on BDNF-induced activation of PLCγ

In addition to the Ras-MAPK and PI3-K/Akt signaling cascades, BDNF also activates another major signal transduction pathway involving PLCγ (Huang and Reichardt, 2001). To assess the influence of sublethal levels of Aβ1-42 on the activation of this pathway by BDNF, we determined the amount of Tyr-phosphorylated PLCγ by Western blot analysis, probing with an anti-PLCγ-specific antibody the immunoprecipitate obtained from cell lysates by an anti-phosphotyrosine antibody (Fig. 8 A). BDNF caused a pronounced increase in Tyr-phosphorylated PLCγ, which was not influenced significantly by Aβ1-42 pretreatment.

Figure 8.

Figure 8.

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1-42 at sublethal concentrations does not interfere with the activation of TrkB and PLCγ. A, BDNF-induced phosphorylation of PLCγ at tyrosine residues. Cortical neurons were stimulated with 50 ng/ml BDNF for 10 min. Cell lysates were immunoprecipitated by agarose-linked anti-phosphotyrosine antibodies, and proteins of the washed immunoprecipitates were resolved by SDS-PAGE and subjected to Western blot analysis with a specific anti-PLCγ antibody (P-PLCγ). BDNF-induced PLCγ phosphorylation was not influenced significantly by Aβ1-42 pretreatment; in terms of phosphorylated PLCγ levels obtained in the BDNF-exposed cultures, the estimate in the Aβ1-42-treated cultures was 92 ± 7.1% (5 μm) and 97 ± 7.2% (10 μm) (n = 3). B, Phosphorylation of TrkB was examined via Western blotting with an antibody against TrkB phosphorylated at Tyr490 (P-TrkB). Pretreatment with 10 μm1-42 had no significant influence on the BDNF-induced P-TrkB content; in terms of P-TrkB levels obtained in the BDNF-exposed culture, the estimate in the Aβ1-42-pretreated cells was 94 ± 4.1% (n = 3).

1-42 does not interfere with the BDNF-induced phosphorylation of TrkB receptors

In contrast to Ras and PI3-K, PLCγ binds to and is phosphorylated directly by the activated TrkB receptor (Huang and Reichardt, 2001). Because Aβ1-42 interfered with BDNF activation of the Ras-MAPK and the PI3-K/Akt pathways, which are activated indirectly by TrkB but did not influence the phosphorylation of PLCγ that is activated directly by the receptor, we hypothesized that Aβ1-42 might not have compromised the BDNF-induced activation of the TrkB receptor. Autophosphorylation of TrkB was assessed by Western blotting, using an antibody specific to the phosphorylated Tyr490 residue. BDNF resulted in pronounced autophosphorylation of the TrkB receptor, which was not compromised by pretreatment with Aβ1-42 (Fig. 8B). Thus, the peptide interferes with BDNF-induced signaling at steps downstream of the BDNF receptor.

1-42 at sublethal concentrations interferes with the phosphorylation of docking proteins that mediate the effects of BDNF on intracellular signaling pathways

Our findings showed, therefore, that treatment with sublethal concentrations of Aβ1-42 interferes selectively with BDNF signaling via the MAPK/ERK and PI3-K pathways, but the initial step, the activation of the receptor, is unaffected, whereas the phosphorylation of intermediate members of the relevant PK cascades, such as Raf, MEK, and Akt, is compromised. The activation of the signaling pathways that were affected by Aβ1-42, the PI3-K and Ras-MAPK/ERK pathways, requires interactions of the activated BDNF receptor with docking proteins that, after phosphorylation, mediate the stimulation of the TrkB receptor to the protein kinase cascades. In contrast, the activated TrkB receptor directly binds and phosphorylates PLCγ, and Aβ1-42 did not affect this process (see above). It is possible, therefore, that Aβ1-42 interferes with signal transduction at the level of the docking proteins. We examined the state of Tyr phosphorylation of IRS-1 that activates both PI3-K and, via Grb2/SOS, the Ras-MAPK/ERK pathway as well the phosphorylation of Shc that mediates signaling via Grb2/SOS to Ras. Figure 9 shows that Aβ1-42 caused an ∼50% reduction in the level of the activated IRS-1 and suppressed the tyrosine phosphorylation of the different Shc isoforms.

Figure 9.

Figure 9.

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1-42 treatment decreased the level of BDNF-activated IRS-1 and Shc. A, Pretreatment with 10 μm1-42 for 2 hr resulted in a significant reduction in the BDNF-induced increase in Tyr-phosphorylated IRS-1. IRS-1 was immunoprecipitated with an anti-IRS-1 antibody. The immunoprecipitates were analyzed by Western blotting with anti-phosphotyrosine antibody (top panel) and with anti-IRS-1 antibody (bottom panel). B, Quantification of the effects of pretreatment with 10 μm1-42. Estimates are the mean ± SEM (n = 3) expressed in terms of Tyr-phosphorylated IRS-1 levels obtained in the BDNF-exposed cultures (*p < 0.05, unpaired Student's t test). C, Pretreatment with 10 μm1-42 for 2 hr resulted in a significant reduction in BDNF-induced increase in Tyr-phosphorylated Shc isoforms as analyzed by immunoprecipitation with an Shc antibody, followed by Western blotting with anti-phosphotyrosine antibody (anti-pY; top panel) and with anti-Shc antibody (bottom panel). The isoforms are indicated as a, b, and c (approximate molecular weights, 66, 52, and 46 kDa, respectively). D, Quantification of the effects of pretreatment with 10 μm1-42. Estimates are the mean ± SEM (n = 3) expressed in terms of phosphorylated P-Shc isoform levels obtained in the BDNF-exposed cultures (*p < 0.05, unpaired Student's t test).

1-42 at sublethal concentrations interferes with the protection by BDNF against neuronal apoptosis induced by either DNA damage or deprivation from trophic support

The observations described so far showed that Aβ1-42 at sublethal concentrations interferes selectively with some BDNF-induced signal transduction pathways in cortical neurons. Next we wanted to explore the effect of the Aβ1-42 treatment on one of the important functions of BDNF, namely the selective protection of neurons against certain types of insults. BDNF can protect cortical neurons from apoptosis induced by camptothecin, an inhibitor of DNA topoisomerase-1 that causes DNA damage (Morris and Geller, 1996). It has been reported that the protective effect of BDNF involves the activation of the MAPK signaling pathway (Hetman et al., 1999). Because sublethal concentrations of Aβ1-42 suppressed BDNF-induced activation of this pathway, we hypothesized that the peptide might interfere with BDNF protection from camptothecin-evoked cell death. Cortical neurons were exposed to 5 μm camptothecin for 24 hr after 1 hr of pretreatment with BDNF or vehicle in the presence or absence of 5 μm1-42. Figure 10A shows that camptothecin treatment caused massive cell loss that was reduced markedly by BDNF treatment and that 5 μm1-42 abolished BDNF protection.

Figure 10.

Figure 10.

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1-42 abrogated BDNF protection of cortical neurons from apoptosis induced either by exposure to camptothecin or by deprivation from trophic support. A, Cortical neurons were exposed to 5 μm camptothecin for 24 hr to induce apoptosis. Additions: Control, vehicle of BDNF solution; BDNF, 10 ng/ml; BDNF + A, 10 ng/ml BDNF + 5 μm1-42; A, 5 μm1-42. When Aβ1-42 was added, the cultures were preincubated in the presence of the peptide for 1 hr. Cell viability was assessed by trypan blue exclusion assay; data are the mean ± SE (n = 3). *p < 0.05 (ANOVA, Fisher's PLSD as the post hoc test). B, The serum-free “trophic” medium B27 was removed from cultures, and after a DMEM wash the cultures were incubated for 36 hr in DMEM in the presence or absence of 10 ng/ml BDNF ± 5 μm1-42. When Aβ was added, there was a 1 hr preincubation period in the presence of 5 μm1-42 before the removal of the B27 medium. For comparison, B27 medium was removed from sister cultures but replaced after a DMEM wash with new B27 medium containing the additives as indicated. Cell survival was assayed by MTT assay; data are the mean ± SE (n = 3). *p < 0.05 (ANOVA, Fisher's PLSD as the post hoc test).

Hetman et al. (1999) also have observed that the BDNF neuroprotection against serum deprivation-induced apoptosis is mediated by the PI3-K/Akt pathway. We tested the protective effect of BDNF on cultures that were deprived from the trophic support provided by the B27 medium. Removal of this medium resulted in significant cell loss by 36 hr, which was prevented completely by BDNF treatment (Fig. 10). The positive effect of BDNF again was compromised severely by sublethal concentrations of Aβ1-42.

Discussion

We currently are testing the hypothesis that Aβ peptides interfere with neuronal functions that play important roles in cognition before massive Aβ deposition and overt neurodegenerative changes occur in the brain in AD. To this end we have chosen to examine the effect of Aβ on signal transduction mechanisms that play critical roles in neuronal plasticity. In an earlier study (Tong et al., 2001) we showed that Aβ1-42 at concentrations at which the viability and the morphology of the cortical neurons are not affected suppressed high K+- or NMDA-induced activation of the transcription factor CREB that is known to play a major role in neuronal plastic changes underlying certain cognitive functions (Tully, 1997; Abel and Kandel, 1998). The effect of sublethal Aβ1-42 on Glu receptor activation-induced elevation of P-CREB levels recently has been confirmed by Vitolo et al. (2002), who also found that the suppression involves protein kinase A inactivation and can be overcome by the activation of the enzyme, which is consistent with the fact that CREB can be phosphorylated by many protein kinases.

The suppression by Aβ1-42 of the neuronal activity-induced P-CREB levels also results in a decrease in the transcription of CREB target genes, as demonstrated by the reduction of BDNF expression (Tong et al., 2001), and BDNF has been shown to participate in certain forms of LTP and learning and memory (Thoenen, 2000; Huang and Reichardt, 2001). In the present study we examined the effect of sublethal levels of Aβ1-42 on signal transduction evoked by BDNF, which under our experimental conditions involves the dominant activation of pathways different from those mediating the effects of membrane depolarization and NMDA receptor activation used in our previous study for neuronal stimulation (Tong et al., 2001). Aβ1-42 treatment resulted in a suppression of the BDNF-induced activation of critical transcription factors, such as CREB and Elk-1, and of CRE- as well as SRE-mediated transcriptional activity, suggesting that Aβ at sublethal levels initiates a vicious cycle in which the effect of the decrease in neuronal stimulation-induced trophic factor production is amplified by the suppression of the trophic factor-elicited signaling and may lead to severe interference with neuronal activity-dependent gene expression.

Under our experimental conditions Aβ1-42 did not compromise cell survival; nevertheless, the concentrations (5-10 μm) were relatively high. However, in the AD brain and in culture after Aβ exposure the peptide accumulates on/in the neuronal plasma membrane, where the concentration is unknown, and in the AD brain Aβ realizes even higher concentrations in senile plaques and diffuse deposits. There also are marked differences in sensitivity in vitro, depending on the preparation and the function studied. For example, similar to us, Vitolo et al. (2002) observed that a sublethal concentration of 5 μm1-42 is required to suppress glutamate-stimulated P-CREB levels in dissociated hippocampal cultures, whereas 200 nm1-42 severely impairs LTP in hippocampal slices. Finally, we observed that an oligomer Aβ1-42 preparation interfered with neuronal activity- or BDNF-induced CREB activation at lower concentrations (100-200 nm) compared with the routine Aβ preparation used in our studies (Tong et al., 2001; this work).

The dominant pathways leading to CREB activation after brief stimulation of neurons with BDNF or high K+/NMDA are different and involve primarily the activation of the Ras-MAPK pathway (Iida et al., 2001) or Ca2+ and calmodulin (CaM)-mediated reactions (Deisseroth et al., 1998; Shieh et al., 1998; Tao et al., 1998). CREB phosphorylation at Ser133 also may involve activated Akt (Du and Montminy, 1998), and we observed that Aβ1-42 treatment also interfered with BDNF activation of Akt. Thus, at sublethal concentrations Aβ1-42 interferes with signal transduction at multiple sites. Nevertheless, it seems that the effect of Aβ1-42 is not nonspecific. Not all major signaling pathways were compromised, because the BDNF-induced phosphorylation of PLCγ was not affected significantly by the Aβ1-42 treatment.

This is an important observation, because PLCγ is activated via direct binding to the autophosphorylated Trk receptors (Huang and Reichardt, 2001), and we observed that Aβ1-42 does not interfere with the BDNF-induced activation of TrkB. In contrast, BDNF activation of the MAPK and PI3-K pathways requires adapter complexes for connection to the activated receptor. We hypothesized, therefore, that Aβ1-42 interferes with BDNF signaling at the level of these docking proteins. This was verified by the observation that Aβ1-42 treatment robustly suppresses the BDNF-stimulated level of Tyr-phosphorylated docking proteins IRS-1 and Shc, which after binding to and being phosphorylated by the activated TrkB receptor bind to and activate PI3-K and, via Grb2/SOS, Ras.

In contrast to the present finding of Aβ-induced suppression of the BDNF-elicited activation of the Ras-MAPK pathway, it has been reported that under certain conditions Aβ alone can induce an increase in the basal level of phosphorylated MAPK. Thus, in hippocampal slices Aβ1-42 activates MAPK via coupling to α7 nicotinic acetylcholine receptors (nAChRs) (Dineley et al., 2001). In our cultures no increase in the basal level of phosphorylated ERK or CREB could be detected after exposure to sublethal Aβ1-42 concentrations (Abe and Saito, 2000). Differences in experimental conditions may account for the discrepancy. In the experiments of Dineley et al. (2001) the Aβ-induced increase in the level of phosphorylated MAPK was transient, peaking at 5 min; by 2 hr, which was the Aβ preincubation time used in our studies, the level of phosphorylated MAPK was restored to that in the untreated preparations. Furthermore, in PC12 and SH-SY5Y neuroblastoma cells, Aβ results in a modest activation of Akt probably via oxygen-derived free radicals (Martin et al., 2001; Wei et al., 2002). We observed a similar weak effect of the peptide on Akt activity. Nevertheless, the BDNF-induced massive increase in Akt activity was suppressed severely by the Aβ pretreatment, indicating that the mechanisms underlying the effect of Aβ causing a weak stimulation of Akt and interfering robustly with the massive BDNF activation of Akt are different.

MAPK/ERK activation is involved critically in mechanisms underlying synaptic plasticity, including long-term memory formation via the stimulation of activity-dependent gene expression (Martin et al., 1997; Atkins et al., 1998; Davis et al., 2000). MAPK phosphorylation results in the activation of two parallel signaling routes required for synaptic plasticity-associated transcriptional regulation, namely signaling via MAPK-Rsk2-CREB and MAPK-Elk-1, which target CRE and SRE, respectively, in the promoter regions of the relevant genes (Bonni et al., 1999; Davis et al., 2000). In certain systems PI3-K activation also is required for synaptic plasticity and memory consolidation (Kelly and Lynch, 2000; Lin et al., 2001), and Akt also can activate CREB (Du and Montminy, 1998), which plays an evolutionarily conserved, important role in learning and memory processes (Tully, 1997; Abel and Kandel, 1998). These observations, together with the finding that Aβ1-42 interferes with BDNF-induced transcriptional activity involving the CRE and SRE promoters, are, therefore, consistent with the view that prolonged exposure to sublethal Aβ1-42 concentrations could contribute significantly to the cognitive decline observed in AD via the suppression of MAPK and PI3-K signaling.

In AD the neurons degenerate as the disease progresses by mechanisms possibly also involving apoptosis-related processes (Cotman et al., 1999). Activated caspases and accumulation of caspase cleavage products as well as DNA fragmentation have been detected in postmortem AD brains. These data suggest that, once the AD brain accumulates insults beyond a critical threshold, an apoptotic pathological cascade is initiated (Cotman et al., 1999). The present study shows the potential functional importance of Aβ1-42 at concentrations at which it does not yet cause degenerative changes, by demonstrating the deleterious effect of the peptide on neuronal vulnerability. Hetman et al. (1999) have established that BDNF is able to prevent cell death triggered by both camptothecin-induced DNA damage via a mechanism involving the activated MAPK pathway and by deprivation from trophic support via a PI3-K-mediated mechanism. We confirmed these observations and found that cell death induced by both camptothecin exposure and deprivation from trophic support is ameliorated by BDNF treatment. However, exposure to sublethal concentrations of Aβ, which interferes with the activation of both the MAPK/ERK and the PI3-K pathways, abrogated the effect of BDNF. The increased neuronal vulnerability in the presence of sublethal concentrations of Aβ may be compounded by the progressive accumulation of other risk factors, including reduced BDNF expression (Phillips et al., 1991; Connor et al., 1997; Ferrer et al., 1999; Tong et al., 2001) and increased DNA damage (Mullaart et al., 1990; Su et al., 1997). Therefore, both reduced BDNF levels and reduced BDNF signaling caused by sublethal Aβ could result, in addition to suppression of synaptic plasticity, in enhanced vulnerability, leading to neuronal dysfunction and, over time, degeneration via apoptosis and other pathways in AD.

In summary, we show that sublethal Aβ1-42 interferes with BDNF signaling by suppressing selectively the activation of the Ras-MAPK/ERK and PI3-K/Akt pathways and the activation of critical transcription factors, such as CREB and Elk-1 and transcription mediated by these factors, and that sublethal Aβ1-42 increases neuronal vulnerability. These observations, together with our earlier findings, are consistent with the view that sublethal Aβ may play important roles in AD pathogenesis before the overt manifestation of the disease by interfering with neuronal functions critical for neuronal maintenance and plasticity.

Footnotes

This work was supported by National Institutes of Health Grant RO1-NS040953.

Correspondence should be addressed to Dr. Liqi Tong, Institute for Brain Aging and Dementia, University of California Irvine, Irvine, CA 92697-4540. E-mail: tongl@uci.edu.

Copyright © 2004 Society for Neuroscience 0270-6474/04/246799-11$15.00/0

References

  1. Abe K, Saito H (2000) Amyloid beta neurotoxicity not mediated by the mitogen-activated protein kinase cascade in cultured rat hippocampal and cortical neurons. Neurosci Lett 292: 1-4. [DOI] [PubMed] [Google Scholar]
  2. Abel T, Kandel E (1998) Positive and negative regulatory mechanisms that mediate long-term memory storage. Brain Res Brain Res Rev 26: 360-378. [DOI] [PubMed] [Google Scholar]
  3. Atkins CM, Selcher JC, Petraitis JJ, Trzaskos JM, Sweatt JD (1998) The MAPK cascade is required for mammalian associative learning. Nat Neurosci 1: 602-609. [DOI] [PubMed] [Google Scholar]
  4. Bonni A, Brunet A, West AE, Datta SR, Takasu MA, Greenberg ME (1999) Cell survival promoted by the Ras-MAPK signaling pathway by transcription-dependent and -independent mechanisms [comments]. Science 286: 1358-1362. [DOI] [PubMed] [Google Scholar]
  5. Bourtchuladze R, Frenguelli B, Blendy J, Cioffi D, Schutz G, Silva AJ (1994) Deficient long-term memory in mice with a targeted mutation of the cAMP-responsive element-binding protein. Cell 79: 59-68. [DOI] [PubMed] [Google Scholar]
  6. Burdick D, Soreghan B, Kwon M, Kosmoski J, Knauer M, Henschen A, Yates J, Cotman C, Glabe C (1992) Assembly and aggregation properties of synthetic Alzheimer's A4/β-amyloid peptide analogs. J Biol Chem 267: 546-554. [PubMed] [Google Scholar]
  7. Causing CG, Gloster A, Aloyz R, Bamji SX, Chang E, Fawcett J, Kuchel G, Miller FD (1997) Synaptic innervation density is regulated by neuron-derived BDNF. Neuron 18: 257-267. [DOI] [PubMed] [Google Scholar]
  8. Chandler LJ, Sutton G, Dorairaj NR, Norwood D (2001) N-methyl d-aspartate receptor-mediated bidirectional control of extracellular signal-regulated kinase activity in cortical neuronal cultures. J Biol Chem 276: 2627-2636. [DOI] [PubMed] [Google Scholar]
  9. Chapman PF, White GL, Jones MW, Cooper-Blacketer D, Marshall VJ, Irizarry M, Younkin L, Good MA, Bliss TV, Hyman BT, Younkin SG, Hsiao KK (1999) Impaired synaptic plasticity and learning in aged amyloid precursor protein transgenic mice. Nat Neurosci 2: 271-276. [DOI] [PubMed] [Google Scholar]
  10. Connor B, Young D, Yan Q, Faull RL, Synek B, Dragunow M (1997) Brain-derived neurotrophic factor is reduced in Alzheimer's disease. Brain Res Mol Brain Res 49: 71-81. [DOI] [PubMed] [Google Scholar]
  11. Cotman CW, Ivins KJ, Anderson AJ (1999) Apoptosis in Alzheimer disease. In: Alzheimer disease, Ed 2 (Terry RD, Katzman R, Bick KL, Sisodia SS, eds), pp 347-358. Philadelphia: Lippincott, Williams and Wilkins.
  12. Datta SR, Brunet A, Greenberg ME (1999) Cellular survival: a play in three Akts. Genes Dev 13: 2905-2927. [DOI] [PubMed] [Google Scholar]
  13. Davis S, Vanhoutte P, Pages C, Caboche J, Laroche S (2000) The MAPK/ERK cascade targets both elk-1 and cAMP response element-binding protein to control long-term potentiation-dependent gene expression in the dentate gyrus in vivo J Neurosci 20: 4563-4572. [DOI] [PMC free article] [PubMed] [Google Scholar]
  14. Deisseroth K, Heist EK, Tsien RW (1998) Translocation of calmodulin to the nucleus supports CREB phosphorylation in hippocampal neurons. Nature 392: 198-202. [DOI] [PubMed] [Google Scholar]
  15. Dineley KT, Westerman M, Bui D, Bell K, Ashe KH, Sweatt JD (2001) β-Amyloid activates the mitogen-activated protein kinase cascade via hippocampal α7 nicotinic acetylcholine receptors: in vitro and in vivo mechanisms related to Alzheimer's disease. J Neurosci 21: 4125-4133. [DOI] [PMC free article] [PubMed] [Google Scholar]
  16. Du K, Montminy M (1998) CREB is a regulatory target for the protein kinase Akt/PKB. J Biol Chem 273: 32377-32379. [DOI] [PubMed] [Google Scholar]
  17. Ferrer I, Marin C, Rey MJ, Ribalta T, Goutan E, Blanco R, Tolosa E, Marti E (1999) BDNF and full-length and truncated TrkB expression in Alzheimer disease. Implications in therapeutic strategies. J Neuropathol Exp Neurol 58: 729-739. [DOI] [PubMed] [Google Scholar]
  18. Finkbeiner S, Tavazoie SF, Maloratsky A, Jacobs KM, Harris KM, Greenberg ME (1997) CREB: a major mediator of neuronal neurotrophin responses. Neuron 19: 1031-1047. [DOI] [PubMed] [Google Scholar]
  19. Hardy J, Selkoe DJ (2002) The amyloid hypothesis of Alzheimer's disease: progress and problems on the road to therapeutics. Science 297: 353-356. [DOI] [PubMed] [Google Scholar]
  20. Hetman M, Kanning K, Cavanaugh JE, Xia Z (1999) Neuroprotection by brain-derived neurotrophic factor is mediated by extracellular signal-regulated kinase and phosphatidylinositol 3-kinase. J Biol Chem 274: 22569-22580. [DOI] [PubMed] [Google Scholar]
  21. Holcomb L, Gordon MN, McGowan E, Yu X, Benkovic S, Jantzen P, Wright K, Saad I, Mueller R, Morgan D, Sanders S, Zehr C, O'Campo K, Hardy J, Prada CM, Eckman C, Younkin S, Hsiao K, Duff K (1998) Accelerated Alzheimer-type phenotype in transgenic mice carrying both mutant amyloid precursor protein and presenilin 1 transgenes. Nat Med 4: 97-100. [DOI] [PubMed] [Google Scholar]
  22. Hsia AY, Masliah E, McConlogue L, Yu GQ, Tatsuno G, Hu K, Kholodenko D, Malenka RC, Nicoll RA, Mucke L (1999) Plaque-independent disruption of neural circuits in Alzheimer's disease mouse models. Proc Natl Acad Sci USA 96: 3228-3233. [DOI] [PMC free article] [PubMed] [Google Scholar]
  23. Hsiao K, Chapman P, Nilsen S, Eckman C, Harigaya Y, Younkin S, Yang F, Cole G (1996) Correlative memory deficits, Aβ elevation, and amyloid plaques in transgenic mice [comments]. Science 274: 99-102. [DOI] [PubMed] [Google Scholar]
  24. Huang EJ, Reichardt LF (2001) Neurotrophins: roles in neuronal development and function. Annu Rev Neurosci 24: 677-736. [DOI] [PMC free article] [PubMed] [Google Scholar]
  25. Iida N, Namikawa K, Kiyama H, Ueno H, Nakamura S, Hattori S (2001) Requirement of Ras for the activation of mitogen-activated protein kinase by calcium influx, cAMP, and neurotrophin in hippocampal neurons. J Neurosci 21: 6459-6466. [DOI] [PMC free article] [PubMed] [Google Scholar]
  26. Ivins KJ, Thornton PL, Rohn TT, Cotman CW (1999) Neuronal apoptosis induced by β-amyloid is mediated by caspase-8. Neurobiol Dis 6: 440-449. [DOI] [PubMed] [Google Scholar]
  27. Kelly A, Lynch MA (2000) Long-term potentiation in dentate gyrus of the rat is inhibited by the phosphoinositide 3-kinase inhibitor, wortmannin. Neuropharmacology 39: 643-651. [DOI] [PubMed] [Google Scholar]
  28. Korte M, Carroll P, Wolf E, Brem G, Thoenen H, Bonhoeffer T (1995) Hippocampal long-term potentiation is impaired in mice lacking brain-derived neurotrophic factor. Proc Natl Acad Sci USA 92: 8856-8860. [DOI] [PMC free article] [PubMed] [Google Scholar]
  29. Lambert MP, Barlow AK, Chromy BA, Edwards C, Freed R, Liosatos M, Morgan TE, Rozovsky I, Trommer B, Viola KL, Wals P, Zhang C, Finch CE, Krafft GA, Klein WL (1998) Diffusible, nonfibrillar ligands derived from Aβ1-42 are potent central nervous system neurotoxins. Proc Natl Acad Sci USA 95: 6448-6453. [DOI] [PMC free article] [PubMed] [Google Scholar]
  30. Li YX, Zhang Y, Lester HA, Schuman EM, Davidson N (1998) Enhancement of neurotransmitter release induced by brain-derived neurotrophic factor in cultured hippocampal neurons. J Neurosci 18: 10231-10240. [DOI] [PMC free article] [PubMed] [Google Scholar]
  31. Lin CH, Yeh SH, Lu KT, Leu TH, Chang WC, Gean PW (2001) A role for the PI-3 kinase signaling pathway in fear conditioning and synaptic plasticity in the amygdala. Neuron 31: 841-851. [DOI] [PubMed] [Google Scholar]
  32. Lue LF, Kuo YM, Roher AE, Brachova L, Shen Y, Sue L, Beach T, Kurth JH, Rydel RE, Rogers J (1999) Soluble amyloid beta peptide concentration as a predictor of synaptic change in Alzheimer's disease. Am J Pathol 155: 853-862. [DOI] [PMC free article] [PubMed] [Google Scholar]
  33. Marshall CJ (1994) MAP kinase kinase kinase, MAP kinase kinase and MAP kinase. Curr Opin Genet Dev 4: 82-89. [DOI] [PubMed] [Google Scholar]
  34. Martin D, Salinas M, Lopez-Valdaliso R, Serrano E, Recuero M, Cuadrado A (2001) Effect of the Alzheimer amyloid fragment Aβ25-35 on Akt/PKB kinase and survival of PC12 cells. J Neurochem 78: 1000-1008. [DOI] [PubMed] [Google Scholar]
  35. Martin KC, Michael D, Rose JC, Barad M, Casadio A, Zhu H, Kandel ER (1997) MAP kinase translocates into the nucleus of the presynaptic cell and is required for long-term facilitation in Aplysia Neuron 18: 899-912. [DOI] [PubMed] [Google Scholar]
  36. Martin SJ, Reutelingsperger CP, McGahon AJ, Rader JA, van Schie RC, LaFace DM, Green DR (1995) Early redistribution of plasma membrane phosphatidylserine is a general feature of apoptosis regardless of the initiating stimulus: inhibition by overexpression of Bcl-2 and Abl. J Exp Med 182: 1545-1556. [DOI] [PMC free article] [PubMed] [Google Scholar]
  37. Martinez A, Alcantara S, Borrell V, Del Rio JA, Blasi J, Otal R, Campos N, Boronat A, Barbacid M, Silos-Santiago I, Soriano E (1998) TrkB and TrkC signaling are required for maturation and synaptogenesis of hippocampal connections. J Neurosci 18: 7336-7350. [DOI] [PMC free article] [PubMed] [Google Scholar]
  38. Minichiello L, Korte M, Wolfer D, Kuhn R, Unsicker K, Cestari V, Rossi-Arnaud C, Lipp HP, Bonhoeffer T, Klein R (1999) Essential role for TrkB receptors in hippocampus-mediated learning. Neuron 24: 401-414. [DOI] [PubMed] [Google Scholar]
  39. Morris EJ, Geller HM (1996) Induction of neuronal apoptosis by camptothecin, an inhibitor of DNA topoisomerase-I: evidence for cell cycle-independent toxicity. J Cell Biol 134: 757-770. [DOI] [PMC free article] [PubMed] [Google Scholar]
  40. Morris JC, Storandt M, McKeel Jr DW, Rubin EH, Price JL, Grant EA, Berg L (1996) Cerebral amyloid deposition and diffuse plaques in “normal” aging: evidence for presymptomatic and very mild Alzheimer's disease. Neurology 46: 707-719. [DOI] [PubMed] [Google Scholar]
  41. Mullaart E, Boerrigter ME, Ravid R, Swaab DF, Vijg J (1990) Increased levels of DNA breaks in cerebral cortex of Alzheimer's disease patients. Neurobiol Aging 11: 169-173. [DOI] [PubMed] [Google Scholar]
  42. Myers SJ, Peters J, Huang Y, Comer MB, Barthel F, Dingledine R (1998) Transcriptional regulation of the GluR2 gene: neural-specific expression, multiple promoters, and regulatory elements. J Neurosci 18: 6723-6739. [DOI] [PMC free article] [PubMed] [Google Scholar]
  43. Naslund J, Haroutunian V, Mohs R, Davis KL, Davies P, Greengard P, Buxbaum JD (2000) Correlation between elevated levels of amyloid β-peptide in the brain and cognitive decline [comments]. JAMA 283: 1571-1577. [DOI] [PubMed] [Google Scholar]
  44. Numakawa T, Matsumoto T, Adachi N, Yokomaku D, Kojima M, Takei N, Hatanaka H (2001) Brain-derived neurotrophic factor triggers a rapid glutamate release through increase of intracellular Ca2+ and Na+ in cultured cerebellar neurons. J Neurosci Res 66: 96-108. [DOI] [PubMed] [Google Scholar]
  45. Oda T, Wals P, Osterburg HH, Johnson SA, Pasinetti GM, Morgan TE, Rozovsky I, Stine WB, Snyder SW, Holzman TF, Krafft GA, Finch CE (1995) Clusterin (apoJ) alters the aggregation of amyloid β-peptide (Aβ1-42) and forms slowly sedimenting Aβ complexes that cause oxidative stress. Exp Neurol 136: 22-31. [DOI] [PubMed] [Google Scholar]
  46. Patterson SL, Abel T, Deuel TA, Martin KC, Rose JC, Kandel ER (1996) Recombinant BDNF rescues deficits in basal synaptic transmission and hippocampal LTP in BDNF knockout mice. Neuron 16: 1137-1145. [DOI] [PubMed] [Google Scholar]
  47. Phillips HS, Hains JM, Armanini M, Laramee GR, Johnson SA, Winslow JW (1991) BDNF mRNA is decreased in the hippocampus of individuals with Alzheimer's disease. Neuron 7: 695-702. [DOI] [PubMed] [Google Scholar]
  48. Pike CJ, Burdick D, Walencewicz AJ, Glabe CG, Cotman CW (1993) Neurodegeneration induced by β-amyloid peptides in vitro: the role of peptide assembly state. J Neurosci 13: 1676-1687. [DOI] [PMC free article] [PubMed] [Google Scholar]
  49. Selkoe DJ (1999) Biology of β-amyloid precursor protein and the mechanism of Alzheimer disease. In: Alzheimer disease, Ed 2 (Terry RD, Katzman R, Bick KL, Sisodia SS, eds), pp 293-310. Philadelphia: Lippincott, Williams and Wilkins.
  50. Shieh PB, Hu SC, Bobb K, Timmusk T, Ghosh A (1998) Identification of a signaling pathway involved in calcium regulation of BDNF expression. Neuron 20: 727-740. [DOI] [PubMed] [Google Scholar]
  51. Snowdon DA, Greiner LH, Markesbery WR (2000) Linguistic ability in early life and the neuropathology of Alzheimer's disease and cerebrovascular disease. Findings from the Nun study. Ann NY Acad Sci 903: 34-38. [DOI] [PubMed] [Google Scholar]
  52. Su JH, Deng G, Cotman CW (1997) Bax protein expression is increased in Alzheimer's brain: correlations with DNA damage, Bcl-2 expression, and brain pathology. J Neuropathol Exp Neurol 56: 86-93. [DOI] [PubMed] [Google Scholar]
  53. Sweatt JD (2001) The neuronal MAP kinase cascade: a biochemical signal integration system subserving synaptic plasticity and memory. J Neurochem 76: 1-10. [DOI] [PubMed] [Google Scholar]
  54. Tao X, Finkbeiner S, Arnold DB, Shaywitz AJ, Greenberg ME (1998) Ca2+ influx regulates BDNF transcription by a CREB family transcription factor-dependent mechanism. Neuron 20: 709-726. [ [DOI] [PubMed] [Google Scholar]; Erratum (1998) 20: 1297] [Google Scholar]
  55. Thoenen H (2000) Neurotrophins and activity-dependent plasticity. Prog Brain Res 128: 183-191. [DOI] [PubMed] [Google Scholar]
  56. Tong L, Thornton PL, Balazs R, Cotman CW (2001) β-Amyloid1-42 impairs activity-dependent cAMP-response element-binding protein signaling in neurons at concentrations in which cell survival is not compromised. J Biol Chem 276: 17301-17306. [DOI] [PubMed] [Google Scholar]
  57. Tully T (1997) Regulation of gene expression and its role in long-term memory and synaptic plasticity. Proc Natl Acad Sci USA 94: 4239-4241. [DOI] [PMC free article] [PubMed] [Google Scholar]
  58. Vitolo OV, Sant'Angelo A, Costanzo V, Battaglia F, Arancio O, Shelanski M (2002) Amyloid β-peptide inhibition of the PKA/CREB pathway and long-term potentiation: reversibility by drugs that enhance cAMP signaling. Proc Natl Acad Sci USA 99: 13217-13221. [DOI] [PMC free article] [PubMed] [Google Scholar]
  59. Walsh DM, Klyubin I, Fadeeva JV, Cullen WK, Anwyl R, Wolfe MS, Rowan MJ, Selkoe DJ (2002) Naturally secreted oligomers of amyloid beta protein potently inhibit hippocampal long-term potentiation in vivo Nature 416: 535-539. [DOI] [PubMed] [Google Scholar]
  60. Wasylyk B, Hagman J, Gutierrez-Hartmann A (1998) Ets transcription factors: nuclear effectors of the Ras-MAP-kinase signaling pathway. Trends Biochem Sci 23: 213-216. [DOI] [PubMed] [Google Scholar]
  61. Wei W, Wang X, Kusiak JW (2002) Signaling events in amyloid β-peptide-induced neuronal death and insulin-like growth factor I protection. J Biol Chem 277: 17649-17656. [DOI] [PubMed] [Google Scholar]
  62. Yankner BA (1996) Mechanisms of neuronal degeneration in Alzheimer's disease. Neuron 16: 921-932. [DOI] [PubMed] [Google Scholar]

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