Background
Due to the capability of NSCs to undergo self-renewal and to differentiate into multiple cell types, NSC-based transplantation has become a potential therapeutic approach in the treatment of neurological disorders such as multiple sclerosis (MS) [
1,
2]. The majority of NSCs come from two areas: the subventricular zone (SVZ) and the subgranular zone of the hippocampus [
3,
4]. Recent reports suggest that, under normal conditions, proliferation and differentiation of NSCs are necessary for neural repair [
5]. However, this function is dramatically reduced in MS, resulting in the breakdown of spontaneous remyelination and neural recovery [
6].
Interleukin-17 (IL-17), an inflammatory cytokine generated by Th17 cells, has been implicated in the development of MS and its animal model, experimental autoimmune encephalomyelitis (EAE) [
7,
8]. By increasing production of several chemokines and cytokines in the central nervous system (CNS) and modulating the inflammatory response, the IL-17/IL-17R pathway plays a critical role in the development of MS [
9,
10]. Although EAE and MS have been considered typical Th1 cell-mediated diseases, growing evidence suggests that Th17 cells play an important role in the effector mechanisms of these, and other, autoimmune diseases [
9,
11‐
13]. Thus, any factor that directly impairs development of Th17 cells, or a deficiency in factors that promote this lineage (IL-1, IL-6, IL-23), consistently abrogates EAE [
14,
15]. IL-17 is the hallmark cytokine of Th17 lineage, which binds to the heteromeric transmembrane receptor, resulting in recruitment of Act1 and formation of a signaling complex that facilitates inflammatory responses [
16]. Mice that lack the IL-17 or IL-17 receptor are less susceptible to EAE induction, and IL-17-specific inhibition attenuates inflammation, suggesting that IL-17 signaling plays a critical role in the effector stage of EAE [
17]. Importantly, increased IL-17 production and mRNA expression have been reported in MS patients with active disease [
18,
19].
However, to date, there have been no reports about the action of IL-17 on NSCs, or on the question whether NSCs express IL-17 receptors. In the current study, we thus address this important question, and investigate the effect of IL-17 on NSC proliferation, differentiation and cell death.
Methods
NSC cultures and differentiation
Mouse NSCs were generated from 14-day-old embryos (E14) from C57Bl/6 mice. Briefly, whole brains of C57BL/6 E14 mouse embryos were harvested under sterile conditions and placed in DMEM medium. After a brief washing with DMEM medium, tissues were cut into 1 mm3 pieces and suspended in 2 ml 0.25% trypsin with EDTA (Invitrogen, NY, USA), mechanically dissociated for 2 min and incubated at 37°C for 30 min. After filtration through a 70 μm cell strainer (BD Bioscience, San Jose, CA), the cell suspension was washed twice with 10 ml DMEM medium. Cells were resuspended in serum-free DMEM/F-12 (Invitrogen, NY, USA) supplied with 2% B27 supplements (Invitrogen, NY, USA), 20 ng/ml epidermal growth factor (EGF, Peprotech, Rocky Hill, NJ, USA) and 20 ng/ml basic fibroblast growth factor (b-FGF, Peprotech, Rocky Hill, NJ), along with 100 IU/ml penicillin and 100 μg/ml streptomycin (Sigma-Aldrich, MI, USA). Cells were then transferred to poly-L-lysine coated 6-well plates (BD Bioscience, San Jose, CA) at a density of 2 × 105 cells/ml and maintained in culture at 37°C. Culture medium was changed every 3 days. Neurospheres were formed after 3-4 days of culture. For passaging, free-floating neurospheres were collected and dissociated with Accutase cell detachment solution (Innovative Cell Technologies, San Diego, CA) into small neurospheres or single cells and re-seeded at a density of 1 × 105 cells/ml in the same medium. NSCs at passage 4-15 were used in all in vitro experiments. To induce NSC differentiation, dissociated single cells or small neurospheres were incubated in stem cell differentiation medium (NSC basal medium plus 10% NSC differentiation supplements, Stemcell Technologies) for 7 to 14 days and processed for immunofluorescence. All animal protocols were approved by the Institutional Animal Care and Use Committee of Thomas Jefferson University, following NIH guidelines.
IL-17R immunostaining
Cells grown on coated cover slips for two days and fixed with 4% paraformaldehyde in PBS (Cellgro Mediatech, USA) were blocked in PBS/0.1% saponin/5% goat serum and incubated with primary antibody at 4°C overnight. Rabbit anti-IL-17R antibody (Santa Cruz, CA, USA) was used to determine IL-17 receptor. Briefly, cells were cultured on slides with stem cell medium, then were washed 2 times with PBS for 5 min, fixed in 3.7% PFA for 10 min at room temperature and washed 3 times with PBS. Blocking was performed in 10% of appropriate serum for 2 hours at room temperature. Cells were then incubated with anti-IL-17R (1:100) overnight at 4°C. After being washed twice in PBS with 0.5% Triton X-100, secondary antibodies were applied for 1 h at room temperature. Cells were then washed, mounted onto Mowiol, and visualized by fluorescence microscopy (Olympus I X-80) with a 20 PlanApo oil immersion objective (1.0 numerical aperture). For visualizing all cells, nuclei were counterstained with DAPI. In this experiment omitting primary antibody was used as control. Images were acquired with a SensiCamQE High Performance CCD Camera.
Real-time PCR
Total RNA was isolated from NSCs in the same culture conditions as those used in immunostaining. RNAs isolated from primary oligodendrocytes (>93% GalC
+) of wild type B6 mice served as IL-17R positive control [
20], and of IL-17R-deficient mice (the Jackson Laboratory) as negative control. For quantitative real-time PCR of IL-17R, specific primers were generated as follows: IL-17RrealF: 5′-AGGTCCAGCCCTTCTTCAGCA-3′, IL-17RrealR: 5′-GCTTGGGAACTGTGGTATTTGA- -GATTA-3′. High Capacity cDNA Reverse Transcription Kit (Invitrogen), RNeasy Mini Kit and QuantiFast SYBR Green PCR Kit (QIAGEN) were used for real-time PCR according to the manufacturer’s instructions.
Analysis of neurosphere growth
To determine the neurosphere volume of stimulated NSCs, these cells were cultured at 200 cells/ml in 96-well plates. These cells were cultured in the presence of IL-17 at different concentrations (0, 5, 10, 25, 50, 100 ng/ml) for 96 hours. NSCs in separate wells were cultured in the presence of TNF-α at 25 ng/ml as positive control, given its cytotoxicity to neural cells [
20], while IL-10 at 50 ng/ml was also used as control, which does not interfere NSC proliferation [
21]. The number of living neurospheres was counted under inverse microscope (ECLIPSE TS-100, Nikon, Japan).
Analysis of cell numbers
To determine the actual number of cells in neurospheres, we did a cell number count after dissociating neurospheres into single cells. Briefly, NSCs were cultured at 1.5 × 10
5 cells/ml in 24 well plates. These cells were cultured in the presence of IL-17 at different concentrations (0, 5, 10, 25, 50, 100 ng/ml) for 96 hours, and in the presence of IL-10 at 50 ng/ml [
21] or TNF-α at 25 ng/ml [
20] as control. Neurospheres were collected, dissociated and cell number was counted under inverse microscope (ECLIPSE TS-100, Nikon, Japan).
MAPK signaling pathway analysis
We then determined p38 MAPK signaling activation in NSCs by western blot. Briefly, cells were cultured at 2 × 105 cells/ml in 6-well plates for 2 days. Two wells were added with IL-17; 2 wells were added with IL-17 and inhibitor of p38 MAPK (SB203580) (Cell Signaling) at 15 mM. Then cells were lysed in lysis buffer (Cell Signaling) supplemented with protease/phosphatase inhibitor cocktail (Cell Signaling). Cell lysates were separated by 12% Tris-Glycine Gels (Novex® 12% Tris-Glycine Mini Gels 1.0 mm, 12-well) and transferred onto Immun-Blot PVDF membrane (Bio-Rad Laboratories). Membranes were blotted with primary antibodies followed by incubation with HRP-conjugated secondary antibodies. The blots were developed by ECL reagents and exposed on HyperFilmTM (Amersham). The following antibodies were used for western blotting: p38 MAPK (D13E1) XP® Rabbit mAb (Cell Signaling), β-Actin (C-4) (Santa Cruz Biotechnology); anti-rabbit IgG HRP-linked antibody (Cell Signaling) and goat anti-mouse IgG-HRP (Santa Cruz Biotechnology).
Analysis of cell death and apoptosis
After incubation at room temperature for 5 min in the dark, cells were trypsinized and resuspended in 50 μL staining buffer containing 100 ng propidium iodide (PI) (Sigma-Aldrich, MI, USA), and then analyzed by flow cytometry. Dead cells were defined as PI positive. Percentages of PI positive cells among cells were calculated.
To assess apoptosis of stimulated cells, NSCs were cultured at 2 × 105 cells/ml in 96 well plates and stimulated with IL-17 (25 ng/ml) for 48 hours. Cells were harvested, then stained with Annexin-V (BD Biosciences, CA, USA), and PI (Sigma-Aldrich, MI, USA) according to the manufacturer’s instructions. Briefly, cells were washed twice with PBS and then resuspended in binding buffer. 5 μl Annexin-V was added to the 100 μl solution in a tube and incubated for 15 min at room temperature in the dark. Cell apoptosis was analyzed by flow cytometry within 1 hour. Apoptotic cells were defined as Annexin-V positive.
Analysis of cytotoxicity
To determine the cytotoxicity of IL-17 on stimulated NSCs, extracellular LDH activity was detected with an LDH Cytotoxicity Detection Kit (Clontech Laboratories, Mountain View, CA) following the manufacturer’s instructions. Briefly, NSCs were cultured at 1 × 105 cells/ml in 96-well plates. These cells were cultured in the presence of IL-17 at different concentrations (0, 5, 10, 25, 50, 100 ng/ml) for 48 hours. The plates were then centrifuged at 250 g for 10 min., and 100 μl of supernatant from each well was transferred into the corresponding well of a 96-well flat-bottom plate. 0.1 ml of freshly prepared Reaction Mixture was added to each well and incubated for up to 30 min at room temperature, protected from light. Absorbance of the samples was measured and the cytotoxicity percentage was calculated according to the manufacturer’s instructions.
Proliferation assay
[3H]-thymidine DNA incorporation was measured in stimulated cells. Briefly, NSCs were cultured at 1.5 × 104 cells/ml in 96-well plates. These cells were cultured in the presence of IL-17 at different concentrations (0, 5, 10, 25, 50, 100 ng/ml) for 48 hours. 1 μCi/well 3H-Thymidine was added to each well. Plates were incubated for 18 hours. 30 μl NaOH 1N solution (Sigma Diagnostics, MO) was added to each well to lyse the cells; then 30 μl hydrochloric acid 1N solution was added to each well to neutralize NaOH (Fisher Scientific, NJ). After supernatant had been thoroughly mixed, radioactivity was measured in a beta-counter.
Immunostaining
Cells grown on coated coverslips and fixed with 4% paraformaldehyde in PBS (Cellgro Mediatech, USA) were blocked in PBS/0.1% saponin/5% goat serum and incubated with primary Abs at 4°C overnight. β-III-tubulin was used as neuron marker; GFAP as an intracellular astrocytic marker; NG2 as oligodendrocyte progenitor cell (OPC) marker and Sox2 as NSC marker. Briefly, cells were cultured on slides with stem cell medium, washed 2 times with PBS for 5 min, fixed in 3.7% PFA for 10 min at room temperature and washed 3 times with PBS. Blocking was performed in 10% appropriate serum for 2 hours at room temperature. Cells were then incubated with anti-β-III-tubulin (1:150); anti-GFAP (1:150); anti-NG2 (1:150) and anti-SOX2 (1:100) overnight at 4°C. After washing twice with PBS containing 0.5% Triton X-100, secondary antibodies were applied for 1 h at room temperature. Cells were then washed, mounted onto Mowiol, and visualized by fluorescence microscopy (Olympus I X-80) with a 20 PlanApo oil immersion objective (1.0 numerical aperture). For visualizing all cells, the nuclei were counterstained with DAPI. In this experiment omitting the primary antibody was used as control. Images were acquired with a SensiCamQE High Performance CCD Camera.
Statistical analysis
Data are presented as the mean ± SE of 3–6 independent experiments, each carried out in triplicate or quadruplicate. Comparisons were analyzed using one-way analysis of variance (ANOVA), followed by a post-hoc Bonferroni's multiple comparison test. Statistical significance was established at p<0.05. The tables and graphs of the original data were produced using GraphPad Prism software version 5.00 for Windows (GraphPad, USA).
Discussion
NSCs are a unique population of cells that exhibit stem cell properties, including self-renewal (production of a large number of progeny) and multipotency (differentiation of the progeny into the three primary CNS phenotypes: neurons, astrocytes and oligodendrocytes) [
22]. NSCs that have been isolated from adult brain can be maintained
in vitro for extended periods of time without losing their proliferation or differentiation potential [
22,
23]. Because NSCs have the ability to support neurogenesis within restricted areas throughout adulthood and can undergo extensive
in vitro expansion, they have been proposed as a renewable source of neural precursors for regenerative transplantation in various CNS diseases, including degenerative disorders, injury and cancer [
24,
25] and EAE [
21,
26,
27]. These cells reached multiple demyelinating areas of the CNS and ameliorated EAE clinically and pathologically to a similar extent when injected either intravenously or intraventricularly [
27]. However, in inflamed foci, such as occur in MS and EAE, which are a hostile microenvironment for NSCs, the migration and proliferation of NSCs are inhibited, resulting in a failure of spontaneous remyelination and neural repair [
28]. It is thus important to identify immune cells and/or proinflammatory mediators that are responsible for this pathogenic outcome.
IL-17A, which has been called IL-17, is the prototypical cytokine of the IL-17 family, which comprises IL-17A-F [
16]. IL-17A and IL-17F trigger signaling via their receptor, a heterodimeric molecule composed of IL-17RA and IL-17RC [
29]. IL-17 activates NFκB signaling and induces several proinflammatory cytokines and chemokines, in particular, CCL20, which can attract CCR6-expressing Th17 cells [
30]. In the CNS, IL-17 activates microglial cells [
31] and induces oligodendrocyte cell death [
20]; it is thus pathogenic in CNS inflammatory demyelination. However, the role of IL-17 signaling in NSCs is not yet known. This question is important given the critical role of these cells in remyelination and neural repair following brain damage. The capacity of NSCs for self-renewal and for generating functional differentiated cells makes them an attractive potential therapeutic tool for the treatment of neurological disorders. Indeed, NSCs have recently emerged as a potential therapeutic approach in the treatment of MS [
2]. In the present study, we demonstrate that IL-17 significantly reduces NSC number by inhibiting the proliferation of these cells, and is thus a novel mechanism underlying the pathogenesis of Th17 cells in the development of CNS inflammatory demyelinating diseases such as MS.
Previous studies have shown that IL-17/IL-17R interactions use TRAF6 to transduce its signal in immune cells [
32], and is a well-studied multi-pathway process of cell death in neural cells [
33]. At the same time, IL-17 mediated activation of JNK1/2 is reported to be involved in cell death [
34,
35]. Moreover, IL-17R has been found to express in oligodendrocytes, the myelinating cells, and adding IL-17 to culture induces significant oligodendrocyte apoptosis [
20]. We hypothesized that NSC apoptosis would be increased after treatment with IL-17. To this end, we tested whether IL-17 had induced NSC apoptosis. Surprisingly, our findings showed that, compared with control, apoptosis in treated NSCs had decreased. Further, we also investigated whether this proinflammatory mediator induced cytotoxicity of these cells, which is an important pathway involved in cell death [
36,
37]. Similarly, IL-17 did not induce lactate dehydrogenase (LDH) release, which is a reliable and simple approach for defining cell death [
38]. Together, these results indicate that the decrease in cell number in treated NSCs resulted from cell proliferation inhibition, not cell death.
The mitogen activated protein kinase (MAPK) family is composed of three main members, including JNK, ERK and p38 MAPK, which can translocate from cytoplasm to nucleus, and induce a series of inflammatory actions in cells [
39]. Among them, the interaction between p38 MAPK and IL-17 is well known for its important role in immunity. For example, IL-17 stimulation induced a high level of proinflammatory cytokine production via the Erk1/2, p38 MAPK, PI3K/Akt, and NF-κB pathways [
40]. On the other hand, activation of p38 MAPK signaling pathway is essential for in vitro and in vivo IL-17 production, and is required for the development and progression of CNS proinflammatory demyelination [
41]. p38 MAPK signaling has also been found to be involved in insufficient NSC proliferation; targeting p38 restored these cells and corrected neuromotor deficits in an ataxia-telangiectasia mouse model [
42]. The importance of p38 MAPK activation in the inhibition of NSC proliferation has also been observed by culturing NSCs with IL-1β, another proinflammatory cytokine that is involved in CNS proinflammatory demyelination [
43]. We demonstrated that the p38 MAPK level in NSCs increased after IL-17 stimulation and that p38 MAPK inhibitor can release the anti-proliferation effect of IL-17. We also showed that the inhibition of NSC proliferation by IL-17 can be partially reversed by p38 MAPK inhibitor. Thus, in addition to its proinflammatory role in the immune system, IL-17 also play a direct role in blocking myelination and neural repair in EAE/MS though the MAPK pathway.
The capacity of NSCs for neural cell differentiation makes these cells a promising potential therapeutic tool for the treatment of nervous system disorders [
1,
2]. Increasing evidence suggests that NSCs go through a process of self-renewal, proliferating and differentiating into the appropriate lineage when inflammatory damage or injury occurs in the nervous system [
44]. To determine the functions of IL-17 on NSC differentiation, we investigated whether IL-17 might hamper the capacity of NSCs to differentiate into neurons, astrocytes and OPCs. While IL-17 stimulation drove NSCs to differentiate into a smaller number of neurons, astrocytes, it resulted in significantly lower numbers of NSCs differentiating into astrocytes and OPCs, cells crucial for remyelination [
21], as well as undifferentiated NSCs. Given that OPCs are the precursor cells of oligodendrocytes, the only myelinating cells in the CNS, reduced OPC differentiation from NSCs could be a potential mechanism of IL-17 pathogenesis in the failure of remyelination in MS/EAE [
45]. Further, given that astrocytes play an important role in the production of neurotrophic factors and support neural repair [
46], reduction of these cells by IL-17 would result in incomplete neural repair after CNS damage. These results, combined with the proinflammatory effect of IL-17 in the peripheral immune system and in the CNS, represent a novel mechanism underlying the failure of spontaneous remyelination and neural repair in the pathogenesis of MS.
Competing interests
The authors declare no competing interests.
Authors’ contributions
The authors have made the following declaration about their contributions: ZL, LZ, GXZ conceived and designed the experiments. ZL, KL performed the experiments. ZL, KL, LZ, QK, YY, HX, AMR, GXZ analyzed the data and wrote the paper. All authors read and approved the final manuscript.