Abstract
Cerebral ischemia stimulates endogenous neurogenesis. However, the functional relevance of this phenomenon remains unclear because of poor survival and low neuronal differentiation rates of newborn cells. Therefore, further studies on mechanisms regulating neurogenesis under ischemic conditions are required, among which ephrin-ligands and ephrin-receptors (Eph) are an interesting target. Although Eph/ephrin proteins like ephrin-B3 are known to negatively regulate neurogenesis under physiological conditions, their role in cerebral ischemia is largely unknown. We therefore studied neurogenesis, brain injury and functional outcome in ephrin-B3−/− (knockout) and ephrin-B3+/+ (wild-type) mice submitted to cerebral ischemia. Induction of stroke resulted in enhanced cell proliferation and neuronal differentiation around the lesion site of ephrin-B3−/− compared to ephrin-B3+/+ mice. However, prominent post-ischemic neurogenesis in ephrin-B3−/− mice was accompanied by significantly increased ischemic injury and motor coordination deficits that persisted up to 4 weeks. Ischemic injury in ephrin-B3−/− mice was associated with a caspase-3-dependent activation of the signal transducer and activator of transcription 1 (STAT1). Whereas inhibition of caspase-3 had no effect on brain injury in ephrin-B3+/+ animals, infarct size in ephrin-B3−/− mice was strongly reduced, suggesting that aggravated brain injury in these animals might involve a caspase-3-dependent activation of STAT1. In conclusion, post-ischemic neurogenesis in ephrin-B3−/− mice is strongly enhanced, but fails to contribute to functional recovery because of caspase-3-mediated aggravation of ischemic injury in these animals. Our results suggest that ephrin-B3 might be an interesting target for overcoming some of the limitations of further cell-based therapies in stroke.
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Introduction
Endogenous neurogenesis persists within distinct areas of the adult mammalian brain such as the subventricular zone (SVZ) [19, 36, 37]. Within this germinal niche, astrocyte-like neural stem cells give rise via rapidly dividing cells to neuroblasts, which migrate along the rostral migratory stream towards the olfactory bulb, where they differentiate into mature neurons [1, 13, 14].
Various physiological and pathological stimuli enhance neurogenesis, among which cerebral ischemia is known to stimulate both proliferation and differentiation of immature neural precursor cells (NPCs) [2, 23, 27, 45]. Although increased neurogenesis under ischemic conditions could contribute to regeneration and restoration, the functional relevance of this phenomenon remains unclear because of poor survival and low neuronal differentiation rates of newborn cells [9, 47]. In order to develop successful neuroregenerative concepts, further knowledge of mechanisms regulating adult neurogenesis under ischemic conditions is urgently needed.
In this context, membrane-bound ephrin proteins interacting via their corresponding ephrin receptors (Eph-receptor) in a bidirectional way [15] have gained increasing attention as signaling molecules associated with neurogenesis. These proteins have diverse roles during prenatal development of the brain with special emphasis on axonal guidance, cell–cell-adhesion and synaptic plasticity [29, 43]. In the adult mammalian brain, ephrin-B2 and ephrin-B3 blockade successfully increased both proliferation and migration of SVZ-derived NPCs under physiological conditions [8, 32]. So far, only one study has analyzed the role of ephrins in the ischemic brain, reporting an increase in proliferation and neuronal differentiation of SVZ-derived NPCs after competitive inhibition of Eph-B2 [44]. In the current study, we show that endogenous neurogenesis is increased after transient focal cerebral ischemia in ephrin-B3 knockout mice without contributing to functional neurological recovery. On the contrary, brain injury in these animals is highly enhanced, involving a caspase-3-associated activation of the signal transducer and activator of transcription 1 (STAT1). We propose that aggravated ischemic brain injury in ephrin-B3 knockout animals is associated with a caspase-3-dependent phosphorylation of STAT1.
Materials and methods
Experimental groups
Experimental procedures were performed according to the European Institutes of Health guidelines for the care and use of laboratory animals and approved by local authorities. Animals were housed under circadian conditions and had free access to food and water. The ephrin-B3 null mice used in the study were kindly provided by Nicholas W. Gale (Regeneron Pharmaceuticals Inc., Tarrytown, NY) and generated as described previously [25].
For all experiments, adult male ephrin-B3 knockout (ephrin-B3–/–) and wild-type mice (ephrin-B3+/+) with an age of 11–14 weeks weighing 25–28 g were used. The total number of animals used was 204. Mice were killed on day 4, 14 and 28 after induction of stroke. Animals used for infarct analysis on day 28 (8 animals each) were also used for behavioral tests. Remaining experimental groups (4- and 14-day survival) consisted of seven animals each. For Western blot, caspase-3 analysis and vessel staining four animals per condition were used. Survival rate was 100% for all experimental groups except for ephrin-B3−/− mice that survived for 28 days, 88.9% for animals used for TTC staining or immunohistochemistry and 80% for animals used for pump implantation experiments. Post-ischemic cell proliferation was analyzed using intraperitoneal (i.p.) injection of 5-bromo-2-deoxyuridine (BrdU; Sigma, Germany) on days 0–3 (4-day survival), days 8–13 (14-day survival) or days 8–18 (28-day survival) with a daily dose of 50 mg/kg bodyweight.
Preparation and cultivation of SVZ-derived neural precursor cells
Preparation and subsequent cultivation of NPCs was done according to a modified protocol from Rietze and Reynolds [33]. NPCs were isolated from the SVZ of 6–8-week-old ephrin-B3−/− and wild-type mice. The SVZ was micro-dissected under stereomicroscopic control (Zeiss, Germany) and minced into small pieces, and then mechanically triturated and dissociated to single cell suspension. Cells were cultured in serum-free basic medium DMEM-F12 (PAA, Austria) supplemented with epidermal growth factor (EGF, 2 μg/ml), basic fibroblast growth factor (bFGF, 2 μg/ml) and penicillin-streptomycin (Invitrogen, Germany). Cells were incubated with 5% CO2 at 37°C. The growth factors were added every 2–3 days, and the cells were passaged by accutase digestion and then re-suspended in pre-warmed conditioned media. Neurosphere passage was done every 7–10 days, and the cells used for experiments were harvested after passage 2–3.
Quantitative neurosphere analysis and proliferation assay
For analysis of neurosphere numbers and neurosphere proliferation, 10,000 NPCs were plated in six-well plates and cultured for 7 days followed by a quantitative analysis of the number of primary neurospheres. The neurospheres were collected with a pipette and transferred to 24-well plates with coverslips coated with 1 mg/ml poly-d-lysine (Sigma, Germany) and 5 μg/ml laminin (Invitrogen, Germany) for immunostaining. The neurospheres were fixed with 4% paraformaldehyde (PFA) for 1 h at 4°C, washed in PBS, blocked for 1 h in blocking solution [0.2% TritonX-100 and 3% bovine serum albumin (BSA) in PBS] and incubated overnight with rabbit anti-phosho-histone-H3 antibody (1:50; Cell Signaling, USA) at 4°C. The neurospheres were then washed and stained with an anti-rabbit Cy3-conjugated secondary antibody (1:200; Jackson ImmunoResearch, USA). For detection of the cell nuclei sections were stained with DAPI (1:20,000; Roth, Germany). The images were acquired using a confocal microscope (Leica TCS SP2) equipped with a 20× objective, and quantitative measurements were performed using MetaMorph software (Molecular Devices, UK).
Neurosphere differentiation assay
For assessment of more subtle differences in cell differentiation, primary neurospheres that had been cultured for 7 days (see above) and neurospheres from passage 3 were gently triturated and plated on 24-well plates (40 cells/μl) containing coverslips coated with 1 mg/ml poly-d-lysine (Sigma, Germany) according to modified protocols [5, 7]. Plating medium consisted of DMEM/F12 medium supplemented with 2% B27 (Invitrogen, Germany), 1% fetal bovine serum (FBS) and penicillin-streptomycin to allow differentiation of cells. For Western blot analysis, cells were lysed (50 mM Tris at pH 8.0, 150 mM NaCl and Triton 1%) on day 7 after plating. Lysates were centrifuged and supernatants were used for SDS-PAGE. Equal amounts of protein (75 μg) were diluted in 6× sample buffer, boiled and loaded onto 10% polyacrylamide gels. Proteins were transferred onto PVDF membranes, which then were immersed in blocking solution [5% milk in TBS-T (0.1% Tween 20 + TBS); 1 h at RT] and incubated with primary antibodies (solved in TBS-T with 1% milk; 18 h at 4°C). The following primary antibodies were used: rabbit polyclonal anti-nestin (1:2,000), rabbit polyclonal anti-glial fibrillary acidic protein (GFAP; 1:10,000), rabbit polyclonal anti-2′,3′-cyclic nucleotide 3′-phosphodiesterase (CNPase; 1 μg/ml) and anti-beta tubulin III (1 μg/ml; all obtained from Abcam, UK). Subsequently, membranes were incubated with a peroxidase-coupled, goat anti-rabbit secondary antibody (1:2,000; Abcam, UK), washed several times, immersed in ECL solution and exposed to ECL-Hyperfilm (Amersham, Germany).
Oxygen-glucose-deprivation (OGD) test
NPCs from both ephrin-B3+/+ and ephrin-B3−/− mice were passaged, and 1,00,000 cells were used for each condition. Before beginning OGD, cell culture medium was substituted by a crystalloid solution that does not contain any glucose (“Thomajodin” plus 1 mM mannitol; DeltaPharm, Germany), and the cells were incubated in a hypoxic chamber (1% O2, 5% CO2 and 94% N2) for 45 min and re-incubated in normal glucose-containing cell culture medium for 24 h. The number of dead cells was counted using a LIVE/DEAD-Viability/Cytotoxicity-Assay kit (Lonza, Switzerland). SVZ-derived NPCs from both ephrin-B3+/+ and ephrin-B3−/− mice that were incubated for 24 h under standard cell culture conditions served as negative controls.
Induction of focal cerebral ischemia
Animals were anesthetized (0.8–1.5% isofluran, 30% O2, remainder N2O), and rectal temperature was maintained at 36.5–37.0°C employing a feedback-controlled heating system. For assessment of blood flow changes, laser Doppler flow (LDF) was recorded during all experiments using a flexible fiberoptic probe (Perimed, Sweden), which was attached to the skull overlying the core region of the middle cerebral artery (MCA) territory (2 mm posterior, 6 mm lateral from bregma). Cerebral ischemia was induced by transient occlusion of the MCA using the intraluminal filament technique as described previously [12]. Briefly, following a midline neck incision, the left common and external carotid artery were isolated and ligated. After placing a microvascular clip (Aesculap, Germany) on the internal carotid artery, a 7–0 silicon coated nylon monofilament (180 μm tip diameter; Doccol, USA) was introduced through an incision into the distal part of the common carotid artery and, after removing the clip, advanced 9 mm distal from the carotid bifurcation for MCA occlusion. To achieve transient ischemia, the monofilament was removed after 30 min (or 20 min in some ephrin-B3−/− mice to achieve similar infarct sizes). LDF recordings continued for 15 min after thread removal to monitor appropriate reperfusion.
Intraventricular pump implantation
Ephrin-B3-Fc ligands (R&D Systems, Germany; 160 μg/ml solved in PBS) were pre-clustered for 2 h at room temperature (RT) (anti-human-Fc ratio 5:1; Jackson Research Laboratories, UK) and applied for intraventricular infusion using a modified protocol from Ricard et al. [32]. Ephrin-B3−/− mice were anesthetized (see above) 1 day before induction of stroke, and cannulae (Brain Infusion Kit; Alzet, USA), which were linked to mini osmotic pumps (volume 200 μl, rate 0.25 μl/h; model Alzet 2004) filled with Ephrin-B3-Fc ligands, were implanted into the left lateral ventricle through a burr hole [31]. Clustered Fc fragments were used as controls. Infusion was performed over a 28-day period, and the animals were killed on day 28 post-stroke for further analysis.
Immunohistochemistry
Animals were i.p. injected with chloralhydrate (420 mg/kg body weight) and transcardiacally perfused with 4% PFA at day 4, 14 or 28 after cerebral ischemia. Brains were removed, post-fixed in PFA and embedded in paraffin, and coronal sections (2 μm) were prepared. Sections were deparaffinized, boiled in 0.2% citrate buffer and incubated with blocking solution (0.3% Triton X-100; 10% normal goat serum in PBS; 1 h, RT). For analysis of BrdU+ or Ki-67+ cells, sections were exposed to blocking solution and subsequently stained with a rat monoclonal anti-BrdU antibody (1:50; 18 h, 4°C; Serotec, Germany), or a rabbit monoclonal anti-Ki-67 antibody (1:100; 18 h, 4°C; Abcam, UK) and a goat anti-rat Alexa 594 (1:500, 1 h; Molecular Probes, Germany), or a donkey anti-rabbit Alexa Fluor 568 (1:400, 1 h; Molecular Probes, Germany) secondary antibody. For differentiation analysis of BrdU+ cells, sections were incubated with a mouse monoclonal anti-BrdU antibody (1:500; Roche, Germany), a goat polyclonal anti-doublecortin antibody (1:50; Santa Cruz Biotechnology, Germany), a rat polyclonal anti-GFAP antibody (1:500; Zymed, Germany) or a rat biotin-conjugated anti-IB4 antibody (1:100; Vector, UK) for 18 h at 4°C. For double staining against BrdU and NeuN or CNPase, a rat monoclonal anti-BrdU antibody (see above) and a mouse monoclonal anti-NeuN antibody (1:200, 18 h, 4°C; Chemicon, UK) or a mouse monoclonal anti-CNPase antibody (1:400; Chemicon, Germany) were used. After washing, sections were incubated for 1 h at RT with the following secondary antibodies: goat anti-mouse Cy-3 (1:400; Dianova, Hamburg, Germany) or goat anti-rat Alexa 594 (1:400; Dianova, Hamburg, Germany) for BrdU staining, goat anti-rat Alexa 488 (1:250; Molecular Probes) or donkey anti-goat Alexa 488 (1:250; Molecular Probes) for GFAP or doublecortin (Dcx) staining, goat anti-mouse Cy-3 (1:100; Jackson Immuno-Research, UK) for CNPase staining and goat anti-mouse Alexa 488 (Molecular Probes, Germany) for NeuN (1:400) staining.
TUNEL staining was performed incubating sections with proteinase K (7 min, 37°C), followed by exposure to the TdT enzyme reaction according to the manufacturer’s manual (Roche, Germany). After several washing steps and exposure to TUNEL blocking solution (20 min, RT), sections were stained with a streptavidin-Alexa594-conjugated secondary antibody (2 h, RT; Molecular Probes).
Quantitative analysis of post-stroke cell injury, cell proliferation and differentiation
Infarct volume analysis was performed on days 4, 14 and 28. Brains were removed and cut into four 2-mm slices. Slices were stained with 2,3,5-triphenyltetrazolium chloride (TTC, 2%), and computer-based analysis of infarct volumes was done using the software Image J as previously described [12]. Assessment of post-ischemic edema formation was performed as the increase of ipsilateral hemispheric volume in comparison to the contralateral hemisphere as described by Wacker et al. [41].
Quantitative analyses for immunohistochemical stainings were performed, defining regions of interest (ROIs) within the SVZ and the basal ganglia (BG). Stereotactic coordinates for quantitative analysis in the SVZ were 0.14 mm anterior, 2–3 mm ventral and 1–1.25 mm lateral from bregma. Cell count analysis within the BG was done at 0.14 mm anterior, 2.5–3.25 mm ventral and 1.5–2.25 mm lateral from bregma. Three sections per animal and ROI were used. Cell death (TUNEL) and neuronal density (NeuN) were assessed within ischemic BG. The number of proliferating cells (BrdU and Ki-67) was determined within the BG and the SVZ. Analysis of cell differentiation was performed using the different markers stated above with subsequent re-calculation as percentages of BrdU+ cells. For assessment of general post-ischemic neuronal differentiation, total numbers of Dcx+ cells and NeuN+/BrdU+ cells within the ischemic BG are given. Data on cell proliferation and differentiation reflect total numbers of counted cells within the SVZ and the BG.
Visualization of anastomotic lines between the anterior cerebral artery (ACA) and the middle cerebral artery territory
In order to exclude increased brain injury of ephrin-B3−/− mice due to differences in macroscopic vessel anatomy, vessel visualization was done following a modified protocol as described previously by us [42]. Non-ischemic ephrin-B3+/+ and ephrin-B3−/− mice were anaesthetized with 1% isoflurane and injected with a lethal dose of papaverine hydrochloride (50 mg/kg BW) intracardially to ensure maximal vasodilatation and vascular filling followed by infusion of 2 ml saline. The thoracic aorta was clipped and the ascending aorta was cannulated. Carbon black solution was prepared with two commercially available inks, i.e., 1.8 ml of Scribtol (Pelikan, Germany) and 0.2 ml of Stempelfarbe (Herlitz, Germany). Five minutes after injection of papavarine, 2 ml of saline was injected into the left ventricle, and immediately afterwards 2 ml of carbon black solution was injected with slight pressure over 40–50 s. After 10 min, animals were decapitated and brains were removed. Photographs of the dorsal and ventral brain surfaces were taken immediately after removal of the brain. Anastomotic lines between ACA and MCA territories were localized by tracing peripheral branches to the points at which vessels were connected. The distance from the midline to the line of anastomosis of the left hemisphere was measured in coronal planes at bregma and at +1 mm from bregma. These levels corresponded to areas where lesion sites were always induced.
Analysis of post-stroke functional deficits
Functional deficits in motor coordination were assessed using both the rota rod and the tightrope test. One day before induction of stroke, all animals were trained before the beginning of the actual tests on days 7, 14, 21 and 28 post-stroke. The rota rod test was performed using an accelerating treadmill for mice (TSE Systems, Germany; 3 cm diameter). Mice were placed on the rotating drum with an accelerating speed of 4–40 rpm. Maximum speed was achieved after 260 s, and maximum testing time was 300 s. The time until animals dropped was registered and statistically analyzed. Using the tightrope test, animals were placed on a 60-cm-long tightrope grasping the string with their forepaws according to a modified protocol from Gerlai et al. [17]. All animals were tested twice per time point. Maximum test time was 60 s, and results were scored from 0 (minimum) to 20 (maximum) according to a validated score (Table 1) depending on the time animals spent on the rope and whether or not they reached the platform.
Caspase-3 assays
Caspase-3 activity was determined using the fluorophore substrate Ac-DEVD-AMC (Biomol, Germany) in brain homogenates of ischemic hemispheres at 1, 2, 3 and 4 h after stroke. Whereas control animals received i.v. injections of 100 μl of 0.2% dimethyl sulfoxide (DMSO), others received 100 μl of the caspase-3 inhibitor z-DEVD.fmk (Biomol, Germany; 500 ng, solved in 0.2% DMSO) at the beginning of the reperfusion. Left hemispheres were complemented with lysis buffer containing 25 mmol/l HEPES, pH 7.5, 1 mM EDTA, 10 mM 1,4-dithiothreitol (Roche, Germany), 0.1% 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS; Sigma-Aldrich, Germany), 10% sucrose, 0.1% Triton X-100 with 10 μg/ml of pepstatin A, aprotinin and leupeptin plus 1 mM phenylmethylsulfonyl fluoride (PMSF; all Sigma-Aldrich, Germany). Samples were homogenized and centrifuged, and supernatants were used for measurements applying 90 μl of samples and 10 μl of substrate (50 μM). Fluorescence (355–460 nm) was detected at 2-min intervals for 20 min with a linear increase between 4–16 min. Caspase-3 activity was re-calculated from the slope (fluorescence units per time) and is given as picomoles of substrate cleaved per milligram of protein per minute based on a standard curve for 7-amino-4-methylcoumarin (AMC; Biomol, Germany). Protein concentration in the supernatant was determined using the Bradford assay.
For analysis of caspase-3-mediated effects on post-ischemic injury, animals received 100 μl of z-DEVD.fmk (500 ng, solved in 0.2% DMSO) or 100 μl of 0.2% DMSO via femoral vein injections at the beginning of the reperfusion. Moreover, animals received additional z-DEVD.fmk or DMSO application via tail vein injection on days 1–3 post-stroke. Thereafter, animals were killed on day 4 and infarct volumes were analyzed.
Detection of phosphorylated STAT1 and STAT3
Phosphorylated STAT1 and STAT3 were measured in brain lysates of ischemic hemispheres at 24 h after stroke using Western blot analysis. Generation of brain lysates and Western blotting procedure were performed as described above. Animals either received z-DEVD.fmk or 0.2% DMSO (see above) at the beginning of the reperfusion. The following primary antibodies were used: rabbit anti-phospho-STAT1 (1:2,000) and rabbit anti-phospho-STAT3 (1:2,500; both obtained from Millipore, Germany). Thereafter, membranes were incubated with a peroxidase-coupled, goat anti-rabbit secondary antibody (1:2,000; Abcam, UK), washed several times, immersed in ECL solution and exposed to ECL-Hyperfilm (Amersham, Germany).
Statistics
All data are given as mean + standard deviation. For comparison between two groups, the two-sided Student's t test was used. For analysis of score data from the tightrope test, however, the non-parametric Wilcoxon-Mann Whitney test was used. A p value of <0.05 was considered to be statistically significant.
Results
In vitro characterization of SVZ-derived NPCs from ephrin-B3–/– mice
NPCs from both mouse strains were first characterized in vitro regarding neurosphere formation, cell proliferation and differentiation as well as behavior after oxygen-glucose deprivation (OGD). Ephrin-B3−/−-derived NPCs showed significantly enhanced primary neurosphere formation and cell proliferation rates compared to controls (Fig. 1a–f). Analysis of cell differentiation in serum containing cell culture medium revealed an increased expression of the neural stem cell/neural progenitor cell marker nestin, the astroglial marker GFAP and the neuronal marker beta-tubulin III in NPCs derived from ephrin-B3−/− mice (Fig. 1g, h). Importantly, protein abundance between primary NPCs (P0) and NPCs from cell culture passage 3 (P3) did not differ within each mouse strain.
To exclude a higher sensitivity of ephrin-B3−/−-derived NPCs to hypoxic-hypoglycemic injury, which is relevant for the functional meaning of post-stroke neurogenesis in vivo, NPCs were exposed to a 45-min OGD and subsequently re-cultivated at standard cell culture conditions (Fig. 1i). OGD induced prominent cell injury in NPCs derived from both mouse strains after 24 h of re-cultivation under standard cell culture conditions. However, we observed no significant difference between cell injury of NPCs that were derived from either ephrin-B3−/− or ephrin-B3+/+ mice.
Analysis of cell proliferation and differentiation after cerebral ischemia
We analyzed post-ischemic cell proliferation in ephrin-B3+/+ and ephrin-B3−/− mice using Ki-67 staining and BrdU staining for up to 4 weeks post-stroke followed by a differentiation analysis of BrdU+ cells. Staining against Ki-67, a marker for current cell proliferation, revealed a significantly higher number of Ki-67+ cells within the ischemic hemisphere of ephrin-B3−/− mice, albeit cell numbers from both mouse strains gradually declined over time (Fig. 2a). In line with this, high numbers of BrdU+ cells were found in the SVZ and the ischemic striatum from both experimental groups, with the vast majority of cells located in the striatum (Fig. 2b–d). Although the number of BrdU+ cells gradually declined over time in both groups, cell numbers were always higher in ephrin-B3−/− mice. No BrdU+ cells were found in the contralateral striatum (data not shown). On the contrary, BrdU+ cells were significantly higher within the contralateral SVZ in ephrin-B3−/− mice at any time point analyzed. We observed, for instance, 7.5 ± 2.4 BrdU+ cells/mm2 in ephrin-B3+/+ and 17.0 ± 3.5 BrdU+ cells/mm2 in ephrin-B3−/− mice on day 28.
Differentiation analysis of proliferating cells was determined using immunohistochemical labeling of neuronal, astroglial and oligodendroglial proteins (Fig. 2e–j). Since BrdU staining at subacute time points essentially reflects activated microglia [11], initial IB4 staining was performed on day 4 post-stroke, revealing 96.4 ± 1.4% in ephrin-B3−/− versus 96.7 ± 3.9% of co-localizations in ephrin-B3+/+ mice in the ischemic striatum. No co-localization of BrdU+ cells with the oligodendroglial marker CNPase was found at any time point analyzed (data not shown). On the contrary, GFAP expression, which was very low on day 4 (data not shown), gradually increased over time in both experimental groups, showing a significantly higher number of BrdU+/GFAP+ cells from 2 weeks on in ephrin-B3−/− mice. Distribution analysis of BrdU+/GFAP+ cells in ephrin-B3+/+ mice revealed 39.6 ± 5.9% of cells located in the SVZ on day 14 and 22.1 ± 4.7% of cells residing in the SVZ on day 28. In ephrin-B3−/− mice, 36.1 ± 3.8% of BrdU+/GFAP+ cells were located in the SVZ on day 14, whereas on day 28 only 16.3 ± 5.2% of cells were found in the SVZ. Immature neuronal differentiation, as assessed by Dcx staining on day 4, was restricted to the SVZ and enhanced in ephrin-B3−/− mice, although the total amount of Dcx+/BrdU+ cells was very low (not shown). Over time, the number of Dcx+/BrdU+ cells, which were from day 14 on also present in the ischemic striatum, gradually increased in both animal strains, but were always significantly higher in ephrin-B3−/− mice. Distribution analysis of BrdU+/Dcx+ cells in ephrin-B3+/+ mice revealed 38.3 ± 7.3% of cells to be found in the SVZ on day 14 and 29.7 ± 3.1% cells in the SVZ on day 28. In ephrin-B3−/− mice, 41.7 ± 7.3% of Dcx+/BrdU+ cells on day 14 and 30.6 ± 3.8% of cells on day 28 were found in the SVZ. Co-localization of BrdU+ cells with the mature neuronal marker NeuN was only observed on day 28 in ephrin-B3−/− mice, where a few newborn cells were seen in the ischemic striatum.
Post-ischemic neurogenesis is enhanced in ephrin-B3–/– mice
Since post-ischemic cell proliferation differed between ephrin-B3+/+ and ephrin-B3−/− mice (Fig. 2a, b), a post-analysis of absolute numbers of Dcx+ and NeuN+/BrdU+ cells was performed, revealing significantly increased absolute numbers of Dcx+ cells in ephrin-B3−/− mice compared to ephrin-B3+/+ mice (Fig. 3a). Beyond day 4 post-stroke, Dcx+ cells were not only restricted to the SVZ (Fig. 3b, c), but also formed typical chain-like clusters within the ischemic striatum (Fig. 3d, e). In ephrin-B3+/+ mice, 35.6 ± 5.4% of Dcx+ cells resided in the SVZ on day 14 and 36.4 ± 6.3% of Dcx+ cells were found in the SVZ on day 28. In ephrin-B3−/− mice, 37.1 ± 7.2% of Dcx+ cells were found in the SVZ on day 14 and 29.2 ± 4.8% of Dcx+ cells were observed in the SVZ on day 28. Moreover, Dcx+ cells were significantly increased in the contralateral SVZ of ephrin-B3−/− mice at any time point analyzed, whereas no Dcx+ cells were found in the contralateral striatum of either animal strain (data not shown). Analysis of absolute numbers of NeuN+/BrdU+ cells at 4 weeks revealed a few scattered cells within the lesion site of ephrin-B3−/− mice but not within the SVZ (Fig. 3f), whereas no NeuN+/BrdU+ cells were detectable in ephrin-B3+/+ mice. These data suggest that endogenous neurogenesis is increased in ephrin-B3−/− mice after induction of cerebral ischemia.
Post-ischemic brain injury is enhanced in ephrin-B3–/– mice
In order to verify whether or not increased neuronal regeneration in ephrin-B3−/− mice was associated with higher resistance to cerebral ischemia, brain injury was analyzed for up to 4 weeks. Surprisingly, ephrin-B3−/− mice revealed significantly enhanced infarct volumes at any time point analyzed (Fig. 4a–g), which was associated with prominent ipsilateral edema formation (Fig. 4h), an increased number of TUNEL+ cells (Fig. 4i–k) and reduced neuronal density in these animals (Fig. 4l–n). Increased post-stroke injury, however, was not due to changes in LDF levels or impaired reperfusion between ephrin-B3−/− and ephrin-B3+/+ mice (data not shown). Even more importantly, there was no significant difference in macroscopic cerebral vessel anatomy as analyzed by visualization of anastomotic lines between the ACA and the MCA territories (Fig. 4o–q) as well as by qualitative analysis of the circle of Willis (Fig. 4r, s). Enhanced brain injury in ephrin-B3−/− mice also resulted in reduced functional recovery with regard to motor coordination as assessed by the rota rod and the tightrope test (Fig. 4t, u). Noteworthily, despite the well-known loss of unilateral movement control in ephrin-B3−/− mice due to re-crossing projections of corticospinal tracts with subsequent simultaneous movement of both hind legs [25], pre-ischemic test performance did not differ between knockout and wild-type mice (Fig. 4t, u).
Elevation of neurogenesis in ephrin-B3−/− mice does not exclusively correlate with the extent of brain injury
Since cerebral ischemia itself triggers neurogenesis, we analyzed whether or not elevated neurogenesis in ephrin-B3−/− mice was due to enhanced ischemic injury in these animals. Therefore, animals were exposed to either 20 min (ephrin-B3−/−) or 30 min of ischemia (ephrin-B3+/+), yielding no significant difference in neuronal density between the two groups (Fig. 5a). On the other hand, analysis of post-ischemic neurogenesis still yielded significantly increased numbers of both Dcx+ and NeuN+/BrdU+ cells within the peri-infarct area of ephrin-B3−/− mice (Fig. 5b, c), which were in the same order as in animals exposed to 30 min of ischemia (Fig. 3a, f).
In order to further support our hypothesis that ephrin-B3 deficiency is crucial for the aforementioned observations made in ephrin-B3−/− mice, knockout animals received continuous intraventricular infusion of soluble ephrin-B3-Fc via mini pumps for as long as 4 weeks. As expected, effects on both brain injury and neurogenesis were reversed by ephrin-B3-Fc-molecules, i.e., animals receiving ephrin-B3-Fc showed less prominent brain injury and reduced post-ischemic neurogenesis than control mice (Fig. 5d–f).
Aggravated ischemic injury in ephrin-B3–/– mice is associated with caspase-3-dependent phosphorylation of STAT1
Since the absence of ephrin-B3 has been shown to induce a caspase-3-mediated cell death under non-ischemic conditions [16], we next analyzed whether or not caspase-3 plays a role in the aggravation of brain injury in ephrin-B3−/− mice. Caspase-3 activity showed a maximum at 2 h post-stroke in both experimental groups, but was significantly higher in ephrinB3−/− mice at this time point and beyond (Fig. 6a). Systemic administration of the caspase-3 inhibitor z-DEVD.fmk resulted in almost completely inhibited enzyme activity in both animal strains (Fig. 6a), but yielded pronounced reduction of brain injury only in ephrin-B3−/− and not in ephrin-B3+/+ mice (Fig. 6b). With consideration of Eph/ephrin signaling having been shown to involve activation of STAT proteins [26], which are thought to have numerous and in part opposing effects in the pathogenesis of stroke [34, 35, 46], protein abundance of phosphorylated STAT1 and STAT3 was analyzed after induction of stroke (Fig. 6c, d). Phosphorylation levels of STAT3 did not differ between the two animal groups at 24 h post-stroke, and treatment with z-DEVD.fmk did not affect protein abundance. On the contrary, protein abundance of phosphorylated STAT1 was significantly increased in ephrin-B3−/− mice as compared to controls. Furthermore, systemic application of the caspase-3 inhibitor yielded significant reduction of STAT1 phosphorylation in ephrin-B3−/− mice, but did not affect STAT1 phosphorylation in wild-type animals. These data suggest that aggravated ischemic brain injury in ephrin-B3−/− mice is associated with a caspase-3-dependent phosphorylation of STAT1.
Discussion
In the present study, we analyzed post-ischemic neurogenesis and cell proliferation, brain injury and functional neurological outcome in ephrin-B3+/+ and ephrin-B3−/− mice. Our study shows that post-stroke neurogenesis is enhanced in ephrin-B3−/− mice without contributing to functional neurological recovery. Rather, brain injury in these animals is significantly enhanced, involving a caspase-3 associated phosphorylation of STAT1.
Eph/ephrin molecules are widely expressed throughout the SVZ, and both the surrounding tissue and Eph/ephrin interactions in these regions have been shown to affect proliferation and apoptosis [8, 20, 24, 32]. The role of ephrin-B3 in adult neurogenesis and neurosphere formation has been described under physiological conditions [32]. However, as neurosphere formation and neurogenesis depend on the species and the age of the animal [4, 5, 40], these results cannot be transferred to our experimental paradigm, which included older animals. In line with Ricard et al. [32] showing an increased self-renewal capacity of NPCs isolated from ephrin-B3−/− mice, we found enhanced neurosphere formation and cell proliferation rates of NPCs derived from ephrin-B3−/− mice, which was associated with significantly increased astroglial and neuronal differentiation rates. Noteworthily, cell differentiation rates were independent of cell passage states, i.e., there was no difference between primary NPCs and NPCs from passage 3.
Although the SVZ itself is not affected by focal cerebral ischemia [12], we further analyzed whether or not NPCs from both mouse strains show different resistance rates against OGD. Importantly, no significant difference was observed, which might be due to the fact that ephrin-B3 is not expressed in the SVZ itself but in the surrounding tissue, which seems to only indirectly affect proliferation and differentiation of NPCs [32].
Cerebral ischemia stimulates endogenous cell proliferation and neurogenesis [2, 21]. Accordingly, stroke-induced high cell proliferation rates within the lesion site of both animal strains. Cell proliferation in the ischemic hemisphere as well as in the contralateral non-ischemic SVZ, however, was always higher in ephrin-B3−/− than in ephrin-B3+/+ mice, suggesting that basal cell proliferation within the germinal niche of ephrin-B3−/− mice is enhanced, as has been previously shown under physiological conditions [32].
A differentiation analysis of proliferating cells revealed a high IB4 abundance of these cells on day 4, reflecting rather activation of microglia than cell differentiation of BrdU+ cells. The decline of cell proliferation over time in both experimental groups therefore most likely reflects a decreased inflammatory response in the ischemic tissue, which is in line with our previous observations where subacute post-stroke cell proliferation was due to microglia activation and not due to enhanced neurogenesis [11]. Astroglial differentiation analysis of proliferating cells revealed an increase over time in both ephrin-B3+/+ and ephrin-B3−/− mice, but were found to be higher in the knockout group from day 14 on. Immature neuronal differentiation of BrdU+ proliferating cells increased over time in both experimental groups, which is consistent with previous reports, where stroke has been shown to increase neuronal differentiation of BrdU+ cells [2, 3, 12, 48]. Nevertheless, immature neuronal differentiation of proliferating cells was always higher in ephrin-B3−/− mice. In spite of this, no newborn mature neurons in the ischemic hemisphere in ephrin-B3+/+ mice were observed, whereas only a few scattered NeuN+/BrdU+ cells were found in ephrin-B3−/− mice 4 weeks post-stroke. In line with this, absolute amounts of newborn neuronal cells, which are more relevant for neuroregeneration, were also significantly increased in ephrin-B3−/− mice. The low neuronal differentiation rates observed in ephrin-B3−/− mice might, however, also be in part due to the limited observation period of 4 weeks with a maximum age of newborn cells of 20 days due to the BrdU-labeling protocol. Although increased neuronal differentiation of BrdU+ cells in ephrin-B3−/− mice has been described before under physiological conditions [32], this is the first time where increased neuronal differentiation in these animals was observed under ischemic conditions. Similarly, enhanced proliferation of SVZ-derived NPCs has recently been described after induction of traumatic brain injury (TBI) in ephrin-B3−/− mice via a p53-dependent pathway [38]. Since stroke and TBI share pathophysiological aspects, including inflammation, further studies have to address the question whether or not p53 is also involved in enhanced proliferation of SVZ-derived NPCs after cerebral ischemia in ephrin-B3−/− mice.
As post-stroke neurogenesis was significantly increased in ephrin-B3−/− mice, we further analyzed whether or not this phenomenon was associated with enhanced resistance to stroke and improved post-stroke recovery. Surprisingly, knockout animals suffered from extensive ischemic brain injury, which was neither due to impaired blood flow nor to differences in vessel anatomy, ultimately resulting in impaired functional recovery of ephrin-B3−/− mice. In this context, the aforementioned enhanced numbers of GFAP+/BrdU+ cells in ephrin-B3−/− animals might rather reflect astroglial proliferation during scar formation than genuine astroglial differentiation of SVZ-derived BrdU+ cells.
As stroke triggers neurogenesis [39], we analyzed whether the enhanced neurogenesis observed in ephrin-B3−/− mice might be due to mere increased brain injury in these animals. Reduction of thread occlusion time in knockout animals resulting in similar infarct sizes compared to wild-type animals did not, however, affect neurogenesis in ephrin-B3−/− mice. Not only was post-ischemic neurogenesis increased when compared to wild-type animals, but was also as high as in ephrin-B3−/− mice that were exposed to longer times of MCA occlusion. In this context, proof of principle experiments using continuous intraventricular infusion of soluble ephrin-B3-Fc-molecules in ephrin-B3−/− mice reversed the aforementioned observations, i.e., both brain injury and neurogenesis were decreased in these animals. As such, enhanced post-ischemic endogenous neurogenesis in ephrin-B3−/− mice does not exclusively depend on the extent of ischemic injury, but is also in part a consequence of intrinsic properties within the knockout mouse.
Although the role of apoptosis and activation of caspase-3 in cerebral ischemia have been studied before, precise apoptotic pathways and demonstration of clinical benefits are still elusive [6, 10, 28]. Interestingly, activation of caspase-3 recently has been shown to occur in the absence of ephrin-B3, resulting in apoptotic cell death under non-ischemic conditions [16]. In the present study, determination of post-stroke caspase-3 activity revealed a significant increase in ephrin-B3−/− mice when compared to controls. Although systemic application of the caspase-3 inhibitor z-DEVD.fmk significantly reduced caspase-3 activity in both animal strains, infarct volumes were only decreased in ephrin-B3−/− but not in ephrin-B3+/+ mice. Noteworthily, ephrin-B3+/+ and ephrin-B3−/− mice developed similar infarct volumes after treatment with the caspase-3 inhibitor. Therefore, caspase-3 activation might be one critical pathway involved in the aggravation of stroke injury in ephrin-B3−/− mice.
As STAT proteins are mediators of Eph/ephrin signaling [26], the abundance of phosphorylated STAT1 and STAT3 was analyzed, resulting in enhanced STAT1 abundance in ephrin-B3−/− mice 24 h post-stroke. On the contrary, no difference in phosphorylated STAT3 abundance between knockout and wild-type animals was observed. Interestingly, systemic application of the caspase-3 inhibitor yielded significantly reduced abundance of phosphorylated STAT1 in ephrin-B3−/− mice, suggesting that a caspase-3-dependent activation of STAT1 might be involved in the aggravation of brain injury in ephrin-B3−/− mice. Nevertheless, the role of STAT proteins in cerebral ischemia and other pathological conditions is still elusive and in part contradictory. STAT proteins are important intracellular mediators of cytokines, among which STAT3 is generally thought rather to induce neuroprotection than cell death [22, 30]. On the contrary, activation of STAT1 has been described to induce both cell injury and neuroprotection under different pathological conditions [18]. We here describe a caspase-3-dependent phosphorylation of STAT1 under ischemic conditions for the first time. In order to verify whether or not aggravation of ischemic injury in ephrin-B3−/− mice is solely dependent on caspase-3-mediated activation of STAT1, further studies are required. However, this beyond the scope of the present work.
In conclusion, our study demonstrates that post-ischemic endogenous neurogenesis is increased in ephrin-B3−/− mice. Ephrin-B3 deficiency, however, also leads to increased brain injury and subsequent impaired neurological recovery, which is associated with a post-ischemic caspase-3-mediated activation of STAT1, pointing towards the notion that cell proliferation, neurogenesis and neurological recovery do not necessarily go in line with each other after stroke. Nevertheless, enhanced proliferation and neuronal differentiation rates of ephrin-B3−/− derived NPCs might be one interesting tool for overcoming the limitations of cell-based therapies in cerebral ischemia, such as poor survival and low differentiation rates of transplanted cells.
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Acknowledgments
We thank Britta Kaltwasser for excellent technical assistance. This work was supported by the DFG Research Center for the Molecular Physiology of the Brain (M.B.), the Internal Research Program of the University of Goettingen (T.R.D.) and the Cluster of Excellence “Macromolecular Complexes” DFG-EXC115 (A.A-P.).
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The authors declare that they have no conflicts of interest.
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Doeppner, T.R., Bretschneider, E., Doehring, M. et al. Enhancement of endogenous neurogenesis in ephrin-B3 deficient mice after transient focal cerebral ischemia. Acta Neuropathol 122, 429–442 (2011). https://doi.org/10.1007/s00401-011-0856-5
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DOI: https://doi.org/10.1007/s00401-011-0856-5