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The Journal of Neuroscience, May 20, 2009, 29(20):6700-6709; doi:10.1523/JNEUROSCI.0233-09.2009
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Cellular/Molecular
A Retrograde Neuronal Survival Response: Target-Derived Neurotrophins Regulate MEF2D and bcl-w
Maria F. Pazyra-Murphy,1,2,3 * Aymeric Hans,1,2,3 * Stephanie L. Courchesne,1,2,3 Christoph Karch,1,2,3 Katharina E. Cosker,1,2,3 Heather M. Heerssen,1,2,3 Fiona L. Watson,1,4 Taekyung Kim,5 Michael E. Greenberg,5 andRosalind A. Segal1,2,3 1Department of Neurobiology, Harvard Medical School, Boston, Massachusetts 02115, 2Departments of Cancer Biology and 3Pediatric Oncology, Dana-Farber Cancer Institute, Boston, Massachusetts 02115, 4Department of Biology and Neuroscience Program, Washington and Lee University, Lexington, Virginia 24450, and 5Department of Neurobiology, Children's Hospital Boston and Harvard Medical School, Boston, Massachusetts 02115
Abstract
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Abstract
Introduction
Survival and maturation of dorsal root ganglia sensory neurons during development depend on target-derived neurotrophins. These target-derived signals must be transmitted across long distances to alter gene expression. Here, we address the possibility that long-range retrograde signals initiated by target-derived neurotrophins activate a specialized transcriptional program. The transcription factor MEF2D is expressed in sensory neurons; we show that expression of this factor is induced in response to target-derived neurotrophins that stimulate the distal axons. We demonstrate that MEF2D regulates expression of an anti-apoptotic bcl-2 family member, bcl-w. Expression of mef2d and bcl-w is stimulated in response to activation of a Trk-dependent ERK5/MEF2 pathway, and our data indicate that this pathway promotes sensory neuron survival. We find that mef2d and bcl-w are members of a larger set of retrograde response genes, which are preferentially induced by neurotrophin stimulation of distal axons. Thus, activation of an ERK5/MEF2D transcriptional program establishes and maintains the cellular constituents of functional sensory circuits.
Introduction
Nerve growth factor (NGF) and brain-derived neurotrophic factor (BDNF) can elicit a wide variety of cellular responses, including proliferation, migration, survival, axonal outgrowth, synapse formation, and plasticity (Segal, 2003; Chao et al., 2006
Neurotrophins were first identified as target-derived trophic factors that bind receptors on axon terminals (Levi-Montalcini and Angeletti, 1968
Here, we consider whether transcriptional responses to neurotrophins depend on location of stimulation. NGF in the skin promotes survival, axonal growth, and differentiation of nociceptive neurons of dorsal root ganglia (DRG) (Chen et al., 1999
Materials and Methods
Cell cultures. Compartmented chamber cultures (Campenot cultures) were prepared as described previously (Heerssen et al., 2004Mass cultures consisting of 2.5 x 105 DRG neurons were grown on laminin-coated p35 culture dishes for 2 d in neurotrophin-enriched (100 ng/ml NGF plus BDNF) media with 0.3 µM AraC, followed by 3 d in 10 ng/ml neurotrophins without AraC. Mass cultures were changed to serum and neurotrophin-free media for 2 h and then stimulated for the indicated time with neurotrophins (100 ng/ml NGF plus BDNF) or vehicle control.
Luciferase assays. African green monkey fibroblast-like (COS-7) cells were maintained in DMEM containing 10% fetal calf serum and 1% penicillin-streptomycin at 37°C, 5% CO2. Firefly luciferase reporter plasmids were transfected into COS cells or DRG neurons using FuGENE 6 (Roche) or by nucleofection (Amaxa Biosystems), respectively, together with TK-pRL, which expresses Renilla luciferase and serves as an internal control. Firefly and Renilla luciferase activity was assessed 72 h after cell transfection. The results shown represent the average of eight independent experiments, with three replicates each.
Plasmids. 3xMRE-Luc, MEF2-VP16 plasmids were described previously (Flavell et al., 2006
Reagents. We used the following antibodies: MEF2D (1:2500 for Western blot and 1:500 for immunostaining; BD Transduction Labs), Bcl-w (1:500; Millipore Bioscience Research Reagents), green fluorescent protein (GFP; 1:1000; Roche), pan-actin (1:1000; Cell Signaling), phospho-ERK5 (1:1000; Cell Signaling), ERK5 (1:500; Cell Signaling), phospho-ERK1/2 (1:1000; Cell Signaling), HA (1:1000; Cell Signaling), Tubulin (1:500; Sigma), phospho-Mef2 (1:500; Abcam); secondary antibodies conjugated to HRP (1:10,000; Bio-Rad), Alexa-488 and Alexa-546 (1:1000; Invitrogen). MEF2D 6066 (1:1000 for Western blot and 1:100 for immunostaining) was developed in the Greenberg lab and generated by injecting antigen (a fragment of MEF2D protein, amino acids 292–514) (Han and Prywes, 1995
Drug treatment. Distal axons and cell bodies of DRG neurons grown in compartmented cultures were treated either with 200 nM K252A (Calbiochem), 10 µM UO126 (Calbiochem), 50 µM LY294002 (Calbiochem), or DMSO vehicle control for 30 min before neurotrophin stimulation.
Real-time quantitative reverse transcription-PCR. RNA was harvested from DRG neurons in compartmented chamber cultures or in mass cultures using the RNAqueous-4PCR kit (Ambion). For in vivo analysis, DRG neurons from E18 rats were dissected, and RNA was extracted using TRIzol (Invitrogen). Reverse transcription (RT) was performed using the cDNA archive kit (Applied Biosystems), according to manufacturer's specifications. Quantitative real-time RT-PCR was performed using Taqman Gene expression assays (Applied Biosystems) to assess the expression of c-fos (Rn02105452_s1), bcl-w (Rn00821025_s1), alsin (Mm00511865_m1), igf-1 (Rn00710306_m1), decorin (Rn01503161_m1), enpep (Rn00573861_m1), and mef2d (Rn00578329_m1). Data were normalized by the expression level of gapdh RNA for each sample (Applied Biosystems). Significance was calculated by z-test.
Protein analysis. Cells were lysed in a nonionic detergent. Protein lysates from 8 to 10 compartmented cultures were pooled, and equal amounts of protein were separated by 7% SDS-PAGE, analyzed by immunoblot, and visualized using the SuperSignal chemiluminescent substrate kit (Pierce).
Immunostaining. For in vitro analysis, compartmented chamber cultures were fixed in 4% paraformaldehyde (PFA) for 20 min, permeabilized in 0.1% TritonX for 10 min, and blocked in 5% normal goat serum and 0.1% TritonX for 60 min. Cultures were incubated overnight at 4°C in MEF2D (1:500) followed by incubation in goat anti-mouse Alexa 546 (1:1000) for 1 h at room temperature.
For in vivo analysis, MEF2D positive cells were counted from postnatal day 0 (P0) bcl-w+/– or bcl-w–/– animals. Animals were killed and fixed in 4% PFA, cryopreserved in 30% sucrose, and 14 µm slices were prepared. Tissue was subjected to antigen retrieval by 10 mM sodium citrate buffer for 15 min at 95°C, followed by 30 min cooling at room temperature. Tissue sections were permeabilized in 0.5% TritonX for 10 min and blocked in 5% normal goat serum and 0.1% TritonX for 60 min. Sections were incubated overnight at 4°C in MEF2D 6066 (1:100) followed by incubation in goat anti-rabbit Alexa 488 (1:1000) for 1 h at room temperature. Three animals of each genotype were used, and 3–6 dorsal root ganglia from each lumbar and cervical region were counted. Significance was calculated by Student's two-tailed t test.
siRNA knockdown. For infection of mass cultures or compartmented cultures with siRNA lentivirus constructs, neurons at 3 and 5 d, respectively, were treated with either control Sh6L3–GFP siRNA or Mef2D–GFP siRNA with polybrene (4 µg/ml) for 48 h. After infection, media was changed to DMEM only for 2 h, and then cells were stimulated with 100 ng/ml NGF plus BDNF or vehicle control for 2 h. Neurons were harvested, and protein levels of MEF2D were analyzed by Western blot. RNA was extracted from cell bodies of compartmented chamber cultures using TRIzol (Invitrogen). Quantitative real-time RT-PCR was performed using Taqman Gene expression assays (Applied Biosystems) to assess the expression of c-fos, bcl-w, and mef2d. Data were normalized by the expression level of gapdh RNA for each sample (Applied Biosystems). Significance was calculated by z-test.
Survival assay. DRG neurons grown in compartmented cultures for 6 d were transferred to serum-free media or to serum-free media supplemented with 100 ng/ml NGF plus BDNF in the distal axon or cell body compartments only. Inhibitors were added to the cell body and distal axon compartments as indicated. We exchanged the media every 12 h to replenish inhibitors and to guard against leakage between compartments. After 72 h, cultures were fixed in 4% paraformaldehyde, and apoptotic cells were visualized using the DeadEnd Fluorometric TdT-mediated dUTP nick end labeling (TUNEL) system kit (Promega), using biotinylated dUTP (5 µM) and Cy3-conjugated avidin (1:1000), and counterstained for 1 min with 4,6-diamidino-2-phenylindole dihydrochloride (DAPI; 1:1000). Each data point represents the mean of five fields per culture from 6 to 12 cultures in 2–6 different experiments scored in a blind manner. Significance was calculated by Student's t test. For in vivo analysis, condensed nuclei using DAPI (1:1000) were counted from P0 bcl-w+/+ or bcl-w–/– animals. Three animals of each genotype were used, and 3–6 dorsal root ganglia from each lumbar and cervical region were counted. Significance was calculated by Student's two-tailed t test.
Animal use. Timed pregnant rats were purchased from Charles River. Bcl-w–/– mice were a generous gift from Grant MacGregor (University of California, Irvine, Irvine, CA) (Ross et al., 1998
Results
MEF2D expression is regulated by neurotrophin stimulation of axons and is important for survival of sensory neurons
Neurotrophin stimulation of distal axons in sensory neurons has previously been shown to increase expression levels of the transcription factors c-fos and c-jun (Watson et al., 1999
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Figure 1. Neurotrophins induce mef2d expression in DRG neurons in response to distal axon stimulation. A, MEF2D protein is detected in vivo in dorsal root ganglia at E18 (lanes 1 and 2 represent 2 separate animals). As a positive control, lysates of neurons over-expressing MEF2VP16 were blotted for MEF2D. B, MEF2D immunostaining of dorsal root ganglia at P0 in vivo. Scale bar, 10 µm. C, Expression of mef2d mRNA in DRG neurons in response to neurotrophin (NT) stimulation. DRG neurons were treated with neurotrophins (100 ng/ml NGF plus BDNF) for 2 h either on distal axons (DA) or on cell bodies (CB). Mef2D mRNA expression is specifically induced by distal axon stimulation and not by cell body stimulation. Expression is compared with DRG neurons treated with vehicle (100 ng/ml BSA). Results represent the mean ± SEM of eight experiments, *p < 0.05. D, Mef2d mRNA expression is upregulated during stimulation of distal axons with NGF alone, BDNF alone, or NGF plus BDNF (NT). Induction of cfos mRNA is shown as a positive control. *p < 0.05. E, MEF2D protein levels were analyzed by Western blotting before and after NT stimulation for 2 h. Normalized relative band density of MEF2D/actin reveal an increase of 21 ± 7% in response to distal axon stimulation.
To determine whether the changes in mef2d mRNA are likely to have functional consequences, we asked whether neurotrophin stimulation also affects the levels of MEF2D protein. As shown in Figure 1E, there is a consistent increase in MEF2D protein in response to neurotrophin stimulation of the distal axons. Furthermore, MEF2D protein is localized to nuclei both before and after neurotrophin stimulation of sensory neurons (supplemental Fig. 1, available at www.jneurosci.org as supplemental material). Together, these data indicate that mef2d mRNA and MEF2D protein are expressed in developing sensory neurons and regulated by neurotrophin stimulation of distal axons and that the protein is appropriately expressed to participate in responses to target-derived neurotrophins.MEF2 family members have been implicated in diverse processes in the nervous system, including survival, proliferation, and synaptic regulation (Mao et al., 1999
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Figure 2. MEF2D is required for survival responses to neurotrophins. A, DRG neurons in culture were infected with lentivirus expressing mef2d–GFP RNAi and cell lysates analyzed by Western blotting with indicated antibodies. Mef2d RNAi (+) results in decreased expression of MEF2D protein levels, whereas a control lentivirus (–) does not. Cerebellar lysate (Cb lysate) was run as a positive control. B, Apoptosis of DRG neurons was analyzed by TUNEL staining. Mef2d RNAi reduces survival of DRG neurons in response to neurotrophins when applied to cell bodies (CB) and blocks survival when applied to distal axons (DA). Results represent the mean ± SEM of five experiments, *p < 0.05. C, Representative images of DRG neuron cell bodies grown in culture and stimulated with neurotrophins or vehicle control on cell bodies or on distal axons. Cells with (mef2d RNAi) or without (control) mef2d reduction are shown. Panels show TUNEL staining (red) and DAPI-stained nuclei in control (top) and in neurons expressing mef2d RNAi (bottom).
The ERK5/MEF2D pathway regulates bcl-w and promotes neuronal survival
We previously found that ERK5 is involved in retrograde signaling and plays an important role in neurotrophin-mediated survival (Watson et al., 2001
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Figure 3. ERK5 regulates MEF2D and promotes survival in response to target derived neurotrophins. A, MEF2D is phosphorylated in response to ERK5 activation. COS cells were transfected with CA–MEK5 and WT–ERK5, or WT–ERK5 alone, and lysates were blotted with an antibody to phospho-MEF2 (p-MEF2). B, MEF2D is phosphorylated in response to cell body stimulation (20 ± 8% increase, p < 0.05) for 20 min. Lysates were blotted with an antibody to phospho-MEF2 and with an antibody to pan-actin as a loading control. C, MEF2D is phosphorylated in response to distal axon stimulation (17 ± 6% increase, p < 0.05) for 2 h. Lysates were blotted with an antibody to phospho-MEF2 and with an antibody to pan-actin as a loading control. D, Neurons were infected with an adenovirus that expresses HA-tagged ERK5-dominant negative form (DN–ERK5), then treated with neurotrophins for 30 min. Compared with uninfected neurons, expression of DN–ERK5 prevents ERK5 phosphorylation without inhibiting ERK1/2 activation. E, ERK5 supports neuronal survival induced by target-derived neurotrophins. Cell apoptosis was measured by TUNEL staining in uninfected neurons and in neurons infected with WT–ERK5 or DN–ERK5 for 2 d. DN–ERK5 blocks survival of neurons that depend on target-derived neurotrophins, whereas DN–ERK5 has a lesser effect on survival supported by cell body stimulation. All data shown are means ± SEM, *p 0.05.
As MEF2D is a transcription factor, we postulate that the ERK5/MEF2D pathway stimulates expression of anti-apoptotic components, such as members of the bcl-2 family. As shown in Figure 4A, the anti-apoptotic gene bcl-w is upregulated by neurotrophin stimulation of distal axons by NGF plus BDNF, NGF alone, or BDNF alone, and not by cell body stimulation. Similarly, when we analyzed Bcl-w protein levels after cell body or distal axon neurotrophin stimulation, Western blotting revealed a significant increase in Bcl-w protein levels (32 ± 5%) after distal axon stimulation, with no increase observed with cell body stimulation (Fig. 4B). The pattern of induction observed for bcl-w resembles that shown for mef2d, in that expression is selectively induced by neurotrophin stimulation of distal axons. We, therefore, tested induction of mef2d and bcl-w after pharmacologic and genetic interventions that prevent activation of the ERK5 pathway, which is needed for retrograde survival responses. Induction of c-fos serves as a positive control in all experiments, as c-fos is induced in response to neurotrophin stimulation of either cell bodies or of distal axons. Both bcl-w and mef2d induction require Trk activation and so are prevented by K252A, an inhibitor of Trk kinase activity; Trk kinase activity is also required for induction of c-fos (Fig. 4C). Like c-fos induction, induction of bcl-w and mef2d are prevented by UO126, a pharmacologic agent that inhibits MEK1 and MEK5 and thus prevents activation of both ERK1/2 and ERK5 (Fig. 4D). In contrast, DN–MEK5, which inhibits activation of ERK5 but not ERK1/2, prevents induction of bcl-w and mef2d but does not affect c-fos. We postulate that ERK5 acts by regulating MEF2D activity. Therefore, we asked whether inhibition of MEF2D has the same effect on gene expression as DN–MEK5. As shown, mef2d RNAi prevents induction of bcl-w, but it does not affect induction of c-fos (Fig. 4E). Together, these data indicate that distal axon stimulation by neurotrophins regulates expression of bcl-w by a pathway that involves Trk/ERK5 and MEF2D and that the mechanisms regulating bcl-w and mef2d expression diverge from pathways that regulate c-fos.
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Figure 4. Target-derived neurotrophins induce bcl-w and mef2d expression in compartmented cultures by a Trk-dependent ERK5/MEF2 pathway. A, Expression of bcl-w mRNA in response to neurotrophin stimulation. DRG neurons were treated with neurotrophin (NT = 100 ng/ml NGF plus BDNF) for 2 h either on distal axons (DA) or on cell bodies (CB). Bcl-w mRNA expression is specifically induced by distal axon stimulation and not by cell body stimulation. Bcl-w mRNA is also upregulated during distal axon stimulation with NGF or BDNF alone. All data show mean ± SEM, *p < 0.05. B, Compartmented cultures were stimulated at cell bodies (CB) or distal axons (DA) for 8 h with neurotrophins. Cell body lysates were analyzed by Western blotting for Bcl-w (recombinant-Bclw was the positive control). DA stimulation leads to an increase in Bcl-w protein levels (32 ± 5%). C, The Trk kinase inhibitor K252a or vehicle control was applied to cell bodies and distal axons at 200 nM, a concentration that inhibits phosphorylation of Trk receptors in these neurons. Neurons in compartmented cultures were globally treated or not with K252a, and DA were stimulated with neurotrophins. K252a prevents induction of c-fos, bcl-w and mef2d by target-derived neurotrophins. D, The Erk kinase inhibitor UO126 or vehicle control was applied to cell bodies and distal axons at 50 nM, a concentration that inhibits phosphorylation of ERK kinases. Neurons in compartmented cultures were treated or not with UO126. UO126 prevents bcl-w, mef2d, and c-fos induction by target-derived neurotrophins. Neurons were infected with DN–MEK5 adenovirus for 3 d, then distal axons were stimulated with neurotrophins. DN–MEK5 expression inhibits bcl-w and mef2d mRNA induction but not c-fos induction by target-derived neurotrophins. E, Lentivirus expressing mef2d RNAi (M2) inhibits induction of bcl-w and mef2d, but not induction of c-fos, in response to target-derived neurotrophins (C = control lentivirus). All data show means ± SEM, *p < 0.05. F, Bcl-w and mef2d mRNA expression is specifically induced by distal axon stimulation and not by global stimulation (cultures maintained for 5–7 d).
To explore the relationship between retrograde signals and neurotrophin-dependent responses originating from activated receptors in the plasma membrane of the cell soma, we asked whether simultaneous neurotrophin stimulation of distal axons and cell bodies of dorsal root ganglion neurons grown in mass culture induces these retrograde response genes. Global stimulation leads to dramatic upregulation of c-fos; in contrast, mef2d and bcl-w are only induced by localized stimulation of distal axons (Fig. 4F). We find that neurotrophin stimulation of cell bodies only increases mef2d and bcl-w mRNA levels when combined with a second intervention that can activate ERK5 (Turjanski et al., 2007As increases in bcl-w and mef2d in response to neurotrophin stimulation occur at the mRNA level, and induction of bcl-w depends on the transcription factor MEF2D, we postulate that induction of these retrograde response genes is mediated (at least in part) at the transcriptional level. To test this directly, we prepared a bcl-w promoter luciferase construct by fusing the 2.5 kB of upstream sequence from the mouse bcl-w promoter to luciferase. As shown (Fig. 5A), this construct contains one of three conserved consensus MEF2D-binding sites upstream of the start site. When expressed in sensory neurons, the bcl-w-luciferase construct is induced by neurotrophin stimulation of distal axons (Fig. 5B). To determine whether this regulation depends on an ERK5/MEF2D pathway, we analyzed the response of the bcl-w-luciferase construct to constitutive activation of ERK5 or MEF2D in COS cells. Coexpression of constitutively active MEK5 and wild-type ERK5 increases expression of bcl-w-luciferase (Fig. 5C). However, no induction is seen when kinase-inactive MEK5 is expressed together with ERK5. As controls, we assessed the response of a basal promoter and a promoter containing MEF2 response elements (MRE). Although activated MEK5/ERK5 induces expression of bcl-w-luciferase and MRE-luciferase, it does not induce expression of basal constructs. To determine whether bcl-w transcription is also mediated by the ERK5 substrate MEF2, we expressed a constitutively active MEF2 construct (VP16-MEF2) together with bcl-w-luciferase and Renilla luciferase control (Fig. 5D). Constitutively active MEF2 stimulates bcl-w-luciferase and the MRE luciferase but does not induce expression of a basic luciferase construct. Together, these studies indicate that bcl-w transcription can be induced by the ERK5/MEF2D pathway and that relevant response elements are contained in the 2.5 kB region upstream of the bcl-w start site. This may include other promoter elements; for example, two sites that resemble half of a CRE-binding motif are also present in the bcl-w promoter region (–9871 to –9867 and 2048 to 2052, TGACG).
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Figure 5. Bcl-w transcription is ERK5 and MEF2-dependent. A, Schematic of bcl-w 5' region. Sequence and locations of consensus MEF2-binding sites are indicated. The luciferase construct consisted of the 2.5 kB promoter region, followed by the necleotides ATG and luciferase reporter gene. B, Luciferase reporter assay using bcl-w promoter-Luc cotransfected with pTK–Renilla–Luc for normalization. Two days after transfection by nucleofection, neurons were stimulated with neurotrophins for 2 h. Bcl-w-luciferase expression is neurotrophin dependent. C, D, Bcl-w promoter is ERK5 and MEF2 dependent. Middle and right luciferase reporter assay using bcl-w promoter-Luc, 3xMRE-Luc, or basic Luce cotransfected into COS cells with Renilla luciferase and the indicated expression plasmid(s). Three days after transfection, luciferase activity was measured. Data are from three independent experiments, each of which was conducted in triplicate, and show means ± SEM, *p < 0.05.
Bcl-w, and other retrograde response genes, promote neuronal survival
Bcl-w has not previously been shown to play a role in dorsal root ganglia neuron survival. To determine whether Bcl-w is important for survival of these spinal sensory neurons, we analyzed dorsal root ganglia neurons from bcl-w–/– mice. These mice are viable, but males are infertile because of apoptosis in the developing testes (Print et al., 1998
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Figure 6. Bcl-w and other retrograde response genes are important for the survival of DRG sensory neurons. A, Representative images of DAPI staining in dorsal root ganglia from cervical and lumbar regions of the spinal cord in bcl-2+/+ and bcl-w–/– mice. Arrows indicate apoptotic cells. Scale bar, 10 µm. B, In vivo analysis of apoptosis. Bcl-w–/– P0 mice show an increase in cell death compared with WT littermates, in both cervical and lumbar DRGs. The percentage of cells in the DRG with condensed nuclei when visualized by DAPI staining are shown. Three animals of each genotype were used, and 3–6 dorsal root ganglia from each lumbar and cervical region were counted. All data show means ± SEM, *p < 0.0001. C, Survival of bclw–/– sensory neurons in compartmented cultures stimulated with neurotrophin applied to the distal axons (DA) or the cell bodies (CB). DRG neurons were dissected at E14 and seeded in compartmented cultures. Bcl-w–/– neurons are more prone to apoptosis in serum free-media compared with bcl-w+/+ and +/– under all conditions tested, *p < 0.05. D, Retrograde response genes: DRG neurons in compartmented cultures were stimulated with NGF and BDNF or vehicle applied either to DA or the cell bodies (CB), for 2 h. RNA was prepared and expression of decorin, alsin, enpeptidase, mef2d, HSF-1, IGF-1, bcl-w, and c-fos were assessed by quantitative RT-PCR and normalized to gapdh in the same sample. Fold induction was measured by comparing normalized level of expression in neurotrophin-treated/vehicle-treated cells for four experiments each involving five cultures for each condition (DA shown first in black). Statistical analysis by z-test, **p
As MEF2D regulates bcl-w and thereby promotes survival, we predict that MEF2D-expressing cells would show decreased survival in the absence of Bcl-w. Therefore, we asked whether the percentage of sensory neurons that express MEF2D is decreased in bcl-w–/– mice. As shown, 30–40% of cervical and lumbar neurons express MEF2D in control neonatal animals. The MEF2D positive cells include neurons that are of various sizes, indicating that this transcription factor is expressed by multiple types of sensory neurons. In bcl-w–/– animals, the pool of MEF2D-expressing neurons is reduced by 23% (percentage of DRG neurons that are MEF2D positive is 37% in control and 28% in bcl-w–/– mice) (supplemental Fig. 3, available at www.jneurosci.org as supplemental material). Thus, in vivo, bcl-w promotes the survival of DRG neurons, and particularly affects MEF2D-expressing cells.We then assessed the survival of dorsal root ganglia sensory neurons from bcl-w–/– mice in compartmented culture conditions. These neurons were grown for 1 week with neurotrophins present in the distal axon compartment, at which point Bcl-w is expressed in wild-type cultures. As shown in Figure 6C, Bcl-w is important for survival of dorsal root ganglia neurons. Indeed, survival of bclw–/– sensory cells is compromised (although not eliminated) at 3 d with, or without, neurotrophins. We were surprised to find that bcl-w–/– neurons exhibit reduced survival during neurotrophin deprivation and under conditions where they are sustained by neurotrophins applied to the cell bodies or distal axons. This differs from the results seen when ERK5 or MEF2D activity is inhibited, in that sensory neurons that depend on target-derived neurotrophins are particularly sensitive to inhibition of ERK5 or MEF2D. Therefore, we asked whether ERK5/MEF2D might regulate additional retrograde response genes as well as bcl-w. Other retrograde response genes might contribute to the differential effect of mef2d RNAi and DN–ERK5 on the survival of neurons supported by neurotrophin stimulation of distal axons or cell bodies. We used quantitative RT-PCR to examine a panel of candidate genes that were induced by neurotrophin stimulation of distal axons in Affymetrix gene arrays, and we identified several genes that are preferentially induced by retrograde signaling (Fig. 6D). The genes identified as retrograde response genes include igf-1 and alsin, which encode proteins that have been implicated in promoting neuronal survival (Boillée and Cleveland, 2004
Discussion
The mechanisms by which target-derived neurotrophic factors initiate and propagate survival signals from nerve terminals to a remote neuronal cell body have been the focus of investigation over many years (Hamburger and Levi-Montalcini, 1949Much of the recent work on long-range signals has focused on the mechanisms by which a signal initiated by an activated receptor at the nerve terminal travels retrogradely to a remote cell body to initiate transcriptional changes (Ginty and Segal, 2002
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Figure 7. Target-derived neurotrophins activate an ERK5/MEF2 transcriptional program to promote survival. A, Neurotrophin binding and Trk activation results in endocytosis of the activated receptor complex. B, The signaling endosome, including downstream messengers, is retrogradely transported by microtubule-dependent dynein motors. C, On reaching the cell body, phosphorylated ERK5 translocates to the nucleus. D, MEF2D is phosphorylated and activated in response to a retrograde ERK5 signal. E, Activated MEF2D initiates transcription of bcl-w, mef2d, and other retrograde response genes (RRGs) to promote survival mediated by target-derived neurotrophins. F, In the case of cell body neurotrophin stimulation, both ERK5 and ERK1/2 are activated; however, expression of bcl-w, mef2d, and other retrograde response genes are not induced. One possible mechanism is through suppression of ERK5 by the ERK1/2 pathway.
Several lines of evidence suggest that transport of signaling endosomes also provides a mechanism by which a neuron can distinguish the location of neurotrophin stimulation and so adjust the nature of its response accordingly. Retinal ganglion cells exhibit increased dendritic arborization in response to BDNF applied at the axon terminals, whereas dendritic arborization is decreased by BDNF stimulation of dendrites within the retina, indicating that the biological response to neurotrophins varies based on location of stimulation (Lom et al., 2002Gene expression programs regulated by ERK5 or other MAPK cascades are specified by the distinct ERK involved, the kinetics of pathway activation and repression, the subcellular localization of the pathway components, and cross talk among distinct kinase cascades (Raman et al., 2007
Our studies have focused on pathways that are required for long-range signaling that promote neuronal survival. We found that ERK5 is particularly important for survival in neurons that depend on target-derived neurotrophins. Neuronal survival is compromised by inhibition of ERK5 activity, and this effect is most dramatic when neurons are supported solely by neurotrophin stimulation of axons. Likewise, MEF2D has a greater role in survival of neurons that depend exclusively on neurotrophin stimulation of the axons. Our data indicate that the anti-apoptotic molecule bcl-w, which is regulated by ERK5 and MEF2D, is important for neuronal survival. However, as survival of Bcl-w–/– sensory neurons is compromised regardless of the location of neurotrophin stimulation, we postulate that ERK5 and MEF2D regulate additional anti-apoptotic retrograde response genes. Intriguingly, igf-1 and alsin are among the putative retrograde response genes (Fig. 6E). IGF-1 promotes neuronal survival by binding to IGF–1R and activating PI3 kinase and Akt (Dudek et al., 1997
Induction of MEF2D by target-derived neurotrophins promotes survival of sensory neurons appropriately connected in a functional circuit, and this is mediated in part by increased transcription of bcl-w. Although our studies have focused on the roles played by ERK5 and MEF2D in neuronal survival in response to target-derived neurotrophins, it is likely that retrograde signaling and retrograde response genes also function in other spatially distinctive responses to neurotrophins. Interestingly, MEF2 transcription factors have been implicated in regulating synaptic connections. Recent studies have shown that a MEF2-dependent transcription program is critical for establishing synaptic morphology and for regulating synapse number (Shalizi and Bonni, 2005
Footnotes
Received Jan. 15, 2009; revised Feb. 24, 2009; accepted March 11, 2009.*M.F.P.-M. and A.H. contributed equally to this work.
A. Hans's present address: French Food Safety Agency, Laboratoire d'Etudes et de Recherches en Pathologie Equine, 14430 Dozulé, France.
C. Karch's present address: Newton, MA 02459.
H. M. Heerssen's present address: Helix Medical Communications, San Mateo, CA 94401.
This work was supported by grants from the National Institutes of Health (NIH) (R.A.S., M.E.G.). We thank Grant MacGregor (University of California, Irvine, Irvine, CA), Susan Corey (The Walter and Eliza Hall Institute of Medical Research, Melbourne, Australia), and Steve Gutkind (NIH) for the generous gifts of reagents. We thank Todd Golub for advice. We thank Erin Berry, Kelly Dakin, Parizad Bilimoria, and Athar Malik for technical assistance.
Correspondence should be addressed to Rosalind A. Segal, Dana-Farber Cancer Institute, 44 Binney Street, Boston, MA 02115. Email: Rosalind_segal{at}dfci.harvard.edu
Copyright © 2009 Society for Neuroscience 0270-6474/09/296700-10$15.00/0
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