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The Journal of Neuroscience, January 25, 2006, 26(4):1269-1274; doi:10.1523/JNEUROSCI.4480-05.2006
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Brief Communications
A Critical Role of Erythropoietin Receptor in Neurogenesis and Post-Stroke Recovery
Peter T. Tsai,1,4 * John J. Ohab,2 * Nathalie Kertesz,1 Matthias Groszer,1 Cheryl Matter,1,3 Jing Gao,1 Xin Liu,1,3,4 Hong Wu,1,4 andS. Thomas Carmichael2 1Departments of Molecular and Medical Pharmacology, 2Neurology, and 3Pathology and Laboratory Medicine, and 4Molecular Biology Institute, University of California at Los Angeles, Los Angeles, California 90095
Abstract
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Abstract
Introduction
Erythropoietin (EPO) is the principal growth factor regulating the production of red blood cells. Recent studies demonstrated that exogenous EPO acts as a neuroprotectant and regulates neurogenesis. Using a genetic approach, we evaluate the roles of endogenous EPO and its classical receptor (EPOR) in mammalian neurogenesis. We demonstrate severe and identical embryonic neurogenesis defects in animals null for either the Epo or EpoR gene, suggesting that the classical EPOR is essential for EPO action during embryonic neurogenesis. Furthermore, by generating conditional EpoR knock-down animals, we demonstrate that brain-specific deletion of EpoR leads to significantly reduced cell proliferation in the subventricular zone and impaired post-stroke neurogenesis. EpoR conditional knockdown leads to a specific deficit in post-stroke neurogenesis through impaired migration of neuroblasts to the peri-infarct cortex. Our results suggest that both EPO and EPOR are essential for early embryonic neural development and that the classical EPOR is important for adult neurogenesis and for migration of regenerating neurons during post-injury recovery.
Key words: erythropoietin; erythropoietin receptor; neurogenesis; ischemia; post-injury recovery; subventricular zone
Introduction
Erythropoietin (EPO) is a cytokine that plays critical roles in hematopoiesis. Both Epo and the classical EpoR are expressed in the nervous system during development and in adult (Digicaylioglu et al., 1995), and their expression levels are upregulated after hypoxic injury (Bernaudin et al., 1999
receptor (
Materials and Methods
Generation of hGFAP-Cre;EpoRfloxp/floxp and hGFAP-Cre;EpoRfloxp/– mice. Generation of Epo–/– and EpoR–/– mice have been described previously (Wu et al., 1995In situ hybridization. Nonradioactive whole-mount mRNA in situ hybridization for Epo and EpoR was performed as described previously (Lee et al., 2001
Stroke model. Stroke was produced in C57BL/6 mice and EpoR conditional knock-down (hGFAP-Cre;EpoRfloxp/floxp) animals (Carmichael, 2005
Immunohistochemistry. Bromodeoxyuridine (BrdU; 50 mg/kg, i.p., in 0.9% saline; Sigma, St. Louis, MO) was given twice daily for 2 d before the animals were killed, or pulse-labeled with a single injection (100 mg/kg, i.p.). At 3, 5, and 7 d after stroke and in control animals (n = 4–6 for each group), tissue was processed for BrdU and doublecortin (DCX) immunostaining (supplemental material, available at www.jneurosci.org). Sections were analyzed with bright-field and epifluorescence microscopy (Leica DMLB) or with laser confocal microscopy (Leica TCS SP MP).
Stereology. Stereological quantification was performed on serial sections through the anterior subventricular zone (SVZ), olfactory bulb, and peri-infarct cortex using unbiased counting with the optical fractionator technique (supplemental material, available at www.jneurosci.org).
Infarct volume. Infarct volume was measured 7 d after stroke in hGFAP-Cre;EpoRfloxp/– and control mice (n = 5 and 4, respectively) (Katsman et al., 2003
Statistics. Post-stroke SVZ counts were tested with factorial ANOVA and Bonferroni’s post hoc testing (Statview 5.0.1; SAS Institute, Cary, NC). Infarct volume, SVZ, and olfactory bulb counts were tested with two-sample t testing assuming unequal variances (Excel; Microsoft, Redmond, WA).
Results
Sequential expression of EpoR and Epo in the developing brain and effects on embryonic development
To understand the function of EPO/EPOR in neurogenesis, Epo and EpoR expression was first determined with in situ hybridization. Whole-mount in situ hybridization of EpoR and Epo in embryonic day 7.5 (E7.5) to E11 embryos shows expression throughout the developing neural tube, with progressive expression in optic placode and forebrain and a delay of 0.5–1 d between EpoR and Epo expression in the same region (supplemental Fig. 1a–f, available at www.jneurosci.org as supplemental material). At E8.5, EpoR expression is confined to the neuroepithelium, a zone of precursors with high proliferation capacity (Fig. 1a, inset). Epo expression is absent at E8.5 (Fig. 1b) but appears by E9.0–E9.5 in the neuroepithelium (Fig. 1d). At E9.5–E10.5, EpoR expression rises in neural crest- and mesenchyme-derived cells (Fig. 1c, e, insets), followed by Epo expression in similar regions 1 d later (Fig. 1f). The temporal and spatial regulation of Epo and EpoR suggests a role for this ligand–receptor pair in early neurogenesis.
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Figure 1. Epo and EpoR expression and neurogenesis defects in null animals. a–f, In situ hybridization of transverse sections with EpoR (a, c, e) or Epo (b, d, f) antisense probes on E8.5, E9.5, and E10.5 embryos. Inset photomicrographs are higher-magnification images from the neuroepithelium (a, c) and neural crest (e). g–l, Epo- (k, l) and EpoR- (g–j) deficient embryos show underdeveloped choroids plexus (i–l) and forebrain (g, h) at E13.5. Con, Control; Mut, mutant.
Both Epo and EpoR null embryos have incomplete neural tube closure at E10.5 (supplemental Fig. 1h, available at www.jneurosci.org as supplemental material), especially in the hindbrain. By E13.5, the neurogenesis defects become more evident, including wavy neural tubes (supplemental Fig. 1j, arrow, available at www.jneurosci.org as supplemental material), underdeveloped telencephalic regions (supplemental Fig. 1j, l, arrowhead, available at www.jneurosci.org as supplemental material). Although no major structures are absent in Epo and EpoR null mice, the mutant brains are consistently smaller and less developed than their littermate controls, particularly in the SVZ of the developing forebrain (Fig. 1h). In addition, the choroid plexus is severely underdeveloped in both null embryos, with a flattened cubiodal epithelium and underdeveloped capillary network (Fig, 1i, l). The identical phenotypes of Epo and EpoR null animals suggest that for early embryonic development, the classical EPOR is essential for EPO action.Generation of EpoR conditional knock-down mice
EPO and EPOR modulate cardiogenesis, vasculogenesis, and neurogenesis (Wu et al., 1999Brain-specific EpoR deletion
EpoRfloxp/floxp mice were crossed with hGFAP-Cre transgenic mice (Zhuo et al., 2001
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Figure 2. Analysis of EpoR conditional knock-down animals. a, PCR. Floxed, WT, and excised alleles ( loxp) are indicated. b, RT-PCR analysis for EpoR expression levels. c, Hematocrit, brain weight, and body weight are unchanged in the mutants. Error bars indicate SDs. d, Cresyl violet sections from control (left) and mutant (right) animals. The bottom panels show higher-magnification views of the boxed areas. Con, Control; Mut, mutant.
Neural-specific EpoR knockdown leads to reduced cell proliferation in the SVZ
Exogenous EPO promotes proliferation, survival, and neuronal differentiation of neural stem cells in vitro (Ling et al., 1998
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Figure 3. Quantification of BrdU labeling in the SVZ. a, Cresyl violet section. The rectangle shows the location of b–g. b–g, BrdU-labeled cells in control (b, d, f) and EpoR conditional knock-down (c, e, g) animals in non-stroke (b, c), 3 d after stroke (d, e), and 7 d after stroke (f, g) are shown. Scale bar, 50 µm. h, i, The graphs show quantifications of BrdU-labeled cells (h) and SVZ volume before and after stroke (i). *p 0.004; #p
EPOR is not essential for protecting neurons from ischemic injury
Previous studies that determined a neuroprotective effect of exogenous EPO (Sakanaka et al., 1998
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Figure 4. EpoR conditional knock-down leads to reduced neuroblast migration. a, b, Cresyl violet sections through the frontal cortex of mutant (a) and control (b) 7 d after stroke. Scale bar, 500 µm. c, Infarct volume 7 d after stroke was quantified. d–g, DCX+ cells in control (d, f) and mutant (e, g). The region within the box in d and e is enlarged in f and g. Scale bars: d, 100 µm; f, 25 µm. h, Stereological quantification of DCX+ cells. #p
EPOR is important for post-stroke neurogenesis
Stroke induces migration of newly born neuroblasts from the SVZ into the area of injury in the first 7–14 d after the insult (Arvidsson et al., 2002The reduction of DCX+ neuroblasts in the cortex of post-stroke EpoR conditional knock-down mice may be attributable to reduced SVZ proliferation, reduced migration to the peri-infarct cortex, or increased cell death in the peri-infarct cortex. To examine proliferation, the number of BrdU+ cells in the SVZ was quantified after stroke (Fig. 3h). Control mice show a significant decrease in BrdU incorporation at day 3 (F(5, 21) = 8.072; p = 0.002) (supplemental Fig. 5d, h, available at www.jneurosci.org as supplemental material), during the period in which DCX+ cells migrate from the SVZ toward the peri-infarct cortex and then a return to baseline at day 7 (Fig. 3f, h). In contrast, the mutant mice have a reduced number of BrdU+ cells and display no change at any time point after stroke (Fig. 3c, e, g, h). The SVZ volume shows similar differences between control and mutant before and after stroke (Fig. 3i). Thus, the mutant SVZ not only has reduced BrdU labeling at baseline but also lacks any significant response to stroke. To determine cell migration and death after stroke, a cohort of DCX cells was labeled by administering BrdU on days 3–5 after stroke and tracking these cells in the peri-infarct cortex on days 5 and 7. In controls, 49 ± 7% of DCX+ cells are BrdU+ at day 5 with further increases to 68 ± 6% by day 7, indicating a continued migration of this cohort of DCX+ cells into the peri-infarct cortex by day 7. In mutants, the percentage of DCX+/BrdU+ cells on day 5 is similar to controls (p = 0.35) but fails to increase by day 7 (55 ± 9%; p = 0.53, MUT day 3 vs day 7). This indicates that there is a failure of continued neuroblast migration into the peri-infarct cortex in EpoR conditional knockdown. To determine whether there is an increase in cell death with EpoR conditional knockdown, the number of terminal deoxynucleotidyl transferase-mediated biotinylated UTP nick end labeling (TUNEL)-positive cells was quantified in the peri-infarct cortex on days 5 and 7 after stroke. There is no significant difference in the number of TUNEL cells in the per-infarct cortex at these two time points (5 d Con, 45 ± 19.6; 5 d Mut, 43.5 ± 11.5; 7 d Con, 42.8 ± 13.3; 7 d Mut, 37.8 ± 14.2; p > 0.63 for all comparisons). Coupled with the significant loss of DCX+r cells in the mutant peri-infarct cortex from days 5–7 (Fig. 4h), these data show that neuroblasts migrate to the peri-infarct cortex in which a subset then undergo cell death. Continued migration of neuroblasts occurs in control animals such that the overall number is maintained, but there is no continued migration in mutant, and the overall number of neuroblasts declines over time.
Discussion
In this study, we provide the first genetic demonstration that EPO and EPOR play essential roles in regulating embryonic and adult neuronal development and function. We demonstrate Epo and EpoR expression during critical periods of neuronal development as well as significantly aberrant neurogenesis in null animals. Then, using a model whereby neuronal EpoR expression is specifically reduced in the brain, we demonstrate a critical role for EPOR in adult neurogenesis and in the migration of newly born neuroblasts to areas of injury. Finally, EpoR conditional knock-down mice display no significant differences in infarct size versus control mice when exposed to stroke, suggesting alternative mechanisms underlying the neuroprotective functions of EPO.EPO/EPOR are required for developmental neurogenesis
The role of EPO in the nervous system extends beyond tissue oxygenation. Epo and EpoR are expressed during critical periods of neuronal development, and Epo and EpoR null animals reveal defects in neurogenesis (Yu et al., 2002EPOR is critical for adult and post-stroke neurogenesis
Exogenous EPO can promote neurogenesis in vitro (Ling et al., 1998Studies in large stroke models in the rat report increased labeling of proliferating cells in the SVZ and migration of newly born neuroblasts from the SVZ to peri-infarct tissue (Arvidsson et al., 2002
Alternative mechanisms for EPO-mediated neuroprotection
Exogenous EPO has been shown to play a neuroprotective role during the ischemic response of the brain by preventing neuronal apoptosis (Sakanaka et al., 1998
Footnotes
Received June 23, 2005; revised Dec. 9, 2005; accepted Dec. 14, 2005.*P.T.T. and J.J.O. contributed equally to this work.
This work was supported in part by the Larry L. Hillblom Foundation and the Nathan Shappell Fund (S.T.C.) and by the Brain Tumor Society Award and the James S. McDonnell Foundation Award (X.L. and H.W.). P.T.T. and C.M. were supported in part by the Medical Scientist Training Program training grant and the Engene V. Cota Robles Award by the Graduate Division through the University of California Office of the President. H.W. is a V Foundation scholar. J.O. was supported by the UCLA Training Program in Neural Repair. We thank Dr. Angus Sinclair (Amgen, Thousand Oaks, CA) and members of our laboratories for helpful comments on this manuscript.
Correspondence should be addressed to either of the following: Dr. Hong Wu, Department of Molecular and Medical Pharmacology, Geffen School of Medicine at University of California at Los Angeles, CHS 23-214, Los Angeles, CA 90095, Email: hwu{at}mednet.ucla.edu; or Dr. S. Thomas Carmichael, Department of Neurology, 635 Charles Young Drive South, University of California at Los Angeles, Los Angeles, CA 90095, scarmichael{at}mednet.ucla.edu
DOI:10.1523/JNEUROSCI.4480-05.2006
Copyright © 2006 Society for Neuroscience 0270-6474/06/261269-06$15.00/0
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