Introduction
Oligodendrocyte precursor cells (OPCs) are widely distributed in the adult central nervous system (CNS). They originate from neural stem cells that line ventricles in discrete regions throughout the brain and spinal cord during embryonic development, then proliferate and migrate through the white matter, and finally differentiate into myelinating oligodendrocytes (OLs) after birth [
1]. Mature OLs wrap axons in layers to form the myelin sheath that protects axons, facilitates the rapid conduction of action potentials, and electrically insulates fibers from one another [
2,
3]. Damage to OLs caused by ischemia, hypoxia, or inflammation can lead to demyelination, which not only influences the transmission of neural signals, but also results in irreversible axonal degeneration. In most cases, OPCs rapidly cluster at lesions after demyelination to proliferate and differentiate into mature OLs, form new myelin sheaths, and wrap exposed axons to achieve functional restoration [
4]. However, remyelination only occurs at an early stage but fails at later stages in many demyelinating diseases such as multiple sclerosis (MS) [
3,
5]. Such a failure of remyelination is mainly attributable to the inability of OPCs to differentiate and mature in demyelinating lesions [
6]. Therefore, promoting the differentiation and maturation of OPCs is crucial to the treatment of these demyelinating diseases.
Shikimic acid (SA), a hydrogenated metabolite of the shikimate pathway, is a precursor for the synthesis of aromatic compounds such as cinnamic acid, flavonoids, alkaloids, anthocyanins, indoles, flavones, alcohol and tannins in plants and microorganisms [
7‐
9]. It is also known as the primary base material for the synthesis of the neuraminidase inhibitor Oseltamivir (Tamiflu®), which is commonly used to treat the H5N1 and A/H1N1 strains of influenza [
10]. Apart from that, researchers have also found that it has anti-cancer effects [
11]. Administration of SA at 200 mg/kg can decrease the expression of pro-inflammatory cytokines induced by lipopolysaccharide and reduce mechanical hyperalgesia in mice [
12]. In addition, SA and its derivative, 3,4-oxo-isopropylidene-shikimic acid, can inhibit platelet aggregation and arterial, venous and cerebral thrombosis as well as promote recovery from ischemic injury [
13,
14]. However, the effects of SA on CNS demyelinating diseases are not clear. In this study, we demonstrated that SA can promote the differentiation and maturation of OPCs and accelerate remyelination, suggesting a potential application in the clinical treatment of demyelinating diseases.
Materials and Methods
Animals and Shikimic Acid
C57BL/6 J mice were purchased from Shanghai SLAC Laboratory Animal Co., Ltd (Shanghai, China), maintained under specific pathogen-free conditions, and used at 6 weeks–8 weeks of age. All animal experiments were performed in adherence with the National Institutes of Health Guidelines on the Use of Laboratory Animals and approved by the Second Military Medical University Committee on Animal Care.
SA was from Sigma-Aldrich (St. Louis, MO), rapidly dissolved in phosphate-buffered saline (PBS) at 100 mg/mL as stock solution (100 ×), and stored in the dark at 4°C. SA was freshly prepared before use.
L-α-lysophosphatidylcholine (LPC) Induced Focal Demyelination in the Dorsal Spinal Cord
Adult (8 weeks–10 weeks old) female C57BL/6 mice were anesthetized by intraperitoneal injection of 3.6% chloral hydrate, and kept on an electric heating pad during the manipulative procedure. Focal demyelination in dorsal spinal cord was induced by LPC (62962, Sigma-Aldrich) as described previously [
15,
16]. Briefly, 1 μL of LPC (0.1% in saline) was injected into the dorsal column at the T11–T12 vertebrae with a micromanipulator. Three days after injection, SA and vehicle were intraperitoneally administered. Mice were anesthetized and sacrificed at 7 days and 14 days after LPC injection, then the spinal cord containing the injection lesion was collected and cut into serial paraffin sections. The demyelinated lesion volume was calculated based on the equation:
V = ∑ demyelinated lesion area × thickness of section [
17].
Experimental Autoimmune Encephalomyelitis (EAE) Model
The EAE model was induced with myelin oligodendrocyte glycoprotein (MOG
35–55) as previously described [
18]. Briefly, female C57BL/6 mice (7 weeks–8 weeks old) were subcutaneously injected with 200 μL of emulsified liquid (mixing ratio, 1:1) consisting of MOG
35–55 (GL Biochem, Shanghai, China) dissolved in 1 × PBS at 1 mg/mL and heat-killed
Mycobacterium tuberculosis (H37Ra strain, Difco, Detroit, MI) mixed evenly in incomplete Freund’s adjuvant (Sigma-Aldrich) at 5 mg/mL. Injections were made at 3 points on the back. The day of injection was recorded as 0 day post-injection (dpi). Pertussis toxin (100 ×) (516561, Calbiochem-EMD Chemicals, San Diego, CA) was dissolved in 1 × PBS and administered intraperitoneally at 0 dpi and 2 dpi. SA was injected intraperitoneally at 15 dpi. Clinical EAE scores were graded daily in a blind manner as follows: 0, no observable symptoms; 1, limp tail; 2, limp tail and partial limb weakness; 3, one hindlimb paralyzed; 4, both hindlimbs paralyzed; 5, moribund or dead.
Primary Oligodendrocyte Progenitor Cell Culture
OPCs were cultured and purified as described previously [
19,
20]. Briefly, mixed glial cells were harvested from P0 rat cortex and cultured in Dulbecco’s modified Eagle’s medium with 10% fetal bovine serum for 10 days at 37°C in a 5% CO
2 incubator. The medium was changed every 3 days. For purification, the flasks were first shaken at 180 rpm for 1 h to remove microglia and at 200 rpm for 16 h with freshly-changed medium at 37°C to collect OPCs. The collected cells were allowed to adhere to uncoated plates for 0.5 h twice to remove contaminating cells. The purified OPCs were collected by gently shaking the plate and seeding them at 5,000 cells/cm
2–50,000 cells/cm
2 on coverslips that had been coated with poly-
D-lysine the previous day. Finally, OPCs were cultured in Neurobasal medium supplemented with 2% B27 for differentiation.
Immunocytofluorescence Staining
Cells on coverslips were fixed in 4% paraformaldehyde (PFA) in 1 × PBS at room temperature for 15 min before washing 3 times with 1 × PBS, followed by permeabilization with 0.1% Triton X-100 for 15 min. Then the cells were incubated overnight at 4°C with primary antibody (myelin basic protein [MBP], 1:50, Chemicon, Temecula, CA; NG2, 1:200, Millipore, Etobicoke, Ontario, Canada). Then the cells were incubated with the corresponding fluorescein isothiocyanate- or tetramethylrhodamine-conjugated secondary antibody (1:l00, Jackson ImmunoResearch, West Grove, PA) and Hoechst 33342 (1:1000) for 1 h at room temperature. Images were captured with a fluorescence microscope (DXM1200; Nikon, Tokyo, Japan).
Immunohistofluorescence Staining
Animals were anesthetized and perfused with 4% PFA. Spinal cord tissue was embedded and sectioned, and post-fixed in PFA overnight at 4°C. Tissue sections were first boiled in 10 mmol/L citrate buffer (pH 6.0) for 20 min at 96°C, then permeabilized with 0.3% Triton X-100 for 30 min and blocked by 5% donkey serum for 1 h. The sections were incubated overnight at 4°C with primary antibody (CC1, 1:100, Millipore; GFAP, 1:200, Sigma; IBA1, 1:200, Abcam, Cambridge, UK), and then with the corresponding secondary antibody for 1 h at room temperature. Last, the samples were examined under a confocal microscope (Leica, Buffalo Grove, IL).
Western Blot Analysis
After treatment with SA or vehicle for 72 h, cells were homogenized in RIPA buffer (Beyotime, Shanghai, China) supplemented with the protease inhibitor phenylmethylsulfonyl fluoride (Beyotime). Then, cell lysates were subjected to Western blotting with a standard protocol as previously described [
18,
19]. The primary antibodies used were anti-MBP (1:500), mTOR (1:3000, CST, Danvers, MA), p-mTOR (1:3000, CST) and the secondary antibodies were horseradish peroxidase conjugated anti-actin (1:50000; Kangchen Biotechnology, Shanghai, China). The primary antibodies were diluted in 1 × TBST and samples were incubated overnight at 4°C. After washing with 1 × TBST, samples were incubated with secondary antibodies for 1 h. The protein bands were analyzed and quantified using Image Lab (Bio-Rad, Hercules, CA).
BrdU Incorporation and TUNEL Assays
BrdU (5-bromo-2-deoxyuridine, 10 μmol/L; Sigma) was added to the medium and incubated for 6 h to label proliferating cells. After fixation in 4% PFA, cells were rinsed three times with 1 × PBS for 5 min, permeabilized with 0.3% Triton X-100 for 10 min, then incubated in 2 N HC1 for 30 min and neutralized in 0.1 mol/L sodium borate for 25 min. Finally, the cells were incubated with primary anti-BrdU (1:100, Sigma) overnight at 4°C as described for Immunocytofluorescence Staining above.
TUNEL assays were carried out with the in situ cell death detection kit, TMR red (12156, Roche, Indianapolis, IN), according to the manufacturer’s instructions. After fixation in 4% PFA, samples were incubated with the TUNEL reaction solution mixture for 1 h at 37°C and then stained with Hoechst 33342 for 5 min at room temperature.
Histological Staining
The spinal cords were isolated from LPC and EAE mice and cut into continuous paraffin sections (4 μm). For Luxol fast blue (LFB) staining, sections were stained with LFB solution overnight in a humid incubator at 60°C, then rinsed with 95% ethanol for 5 min, 0.05% lithium carbonate, and 70% ethanol for 20 s, then washed with water.
For hematoxylin and eosin (H&E) staining, sections were stained with hematoxylin for 3 min–5 min, then rinsed in ethanol with 1% HCl for 10 s and 1% ammonia water, then counterstained with eosin. After dehydration through a series of graded ethanols and cleared with xylene, the sections were mounted in Permount mounting medium (Fisher Scientific, Pittsburgh, PA).
Statistical Analyses
Data are presented as mean ± SD or mean ± SEM from at least three independent experiments unless otherwise indicated. One-way ANOVA with Tukey’s post hoc test was used for multiple groups and Student’s t test for two groups. The EAE model was analyzed using the nonparametric Mann–Whitney U test to compare two groups or the Kruskal–Wallis test with Dunn’s post hoc test to compare four groups. P < 0.05 was considered statistically significant.
Discussion
Generally, remyelination proceeds spontaneously in response to CNS demyelination, and this pathophysiological process depends on the differentiation and maturation of OPCs [
27]. After demyelination, OPCs rapidly switch from the resting to the activated state, followed by recruitment, proliferation, and differentiation into mature OLs. Then, mature OLs form new myelin sheaths to protect axons and restore signal transmission [
4,
28,
29]. Although they remain competent to restore myelin sheaths throughout adulthood, OPCs fail to remyelinate in some demyelinating diseases, such as MS, of which the main pathological features are inflammation-mediated demyelination and multifocal lesions with axonal degeneration [
30]. At present, the therapeutic strategy for MS mainly depends on immunosuppression and immunomodulation to reduce the recurrence rate of relapsing-remitting MS, while there is no effective remedy for progressive MS [
31,
32]. Previous studies have shown that the failure of remyelination in MS is mainly attributed to the inability of differentiation and maturation of OPCs [
6,
33]. Therefore, it is of great importance to seek potential treatments to promote the differentiation and maturation of OPCs.
SA has been shown to protect the neuronal cell line SH-SY5Y against oxidative stimulation which usually occurs under neurodegenerative conditions [
9]. In addition, its derivative, 3,4-oxo-isopropylidene-shikimic acid, has been reported to have a similar protective effect for astrocytes and neurons in a rat model of cerebral ischemic injury [
34]. However, whether SA has a beneficial impact on OPCs is unknown. In the present study, based on the vital function of myelination along with its specificity as a marker of mature OLs, MBP was selected as a target to test the effects of SA on OPC differentiation. SA showed a significant dose-dependent up-regulation of MBP expression. Consistently, the number of MBP-positive mature OLs marked by immunostaining increased remarkably after SA treatment. Meanwhile, SA reduced the number of NG2-positive OPCs. As SA did not affect the proliferation and apoptosis of OPCs, our results suggested that SA specifically promotes the differentiation and maturation of OPCs.
To directly assess the possible application of SA to demyelinating diseases, we assessed the effects of SA on EAE, the most commonly-used animal model for studying MS. We found that SA significantly inhibited the inflammation and demyelination and reduced the number of astrocytes and microglia in the spinal cord, and the overall neurological functional recovery in EAE mice was improved as well. It has been reported that SA inhibits lipopolysaccharide-induced cellular pro-inflammatory cytokines as well as attenuating mechanical hyperalgesia in mice [
8] through inhibiting ERK 1/2 and p38 phosphorylation. We presume that the underlying mechanism of SA in EAE is similar, but this needs further investigation.
Since the pathogenesis of EAE is complex and involves a variety of interactions between the immune and nervous systems [
35] and the demyelination and remyelination occur concurrently, it is difficult to distinguish between the reduction of demyelination and the promotion of remyelination [
17]. In order to further assess the specific effects of SA on remyelination, we introduced a chemical injury model, that is, LPC-induced focal demyelination. In this model, demyelination and remyelination are generated along a reproducible timeline [
36]. Most importantly, the interference of inflammatory factors in EAE can be avoided in the LPC model, which thus can simply and directly reflect the effect of a drug on remyelination [
35]. Our data demonstrated that SA did not affect the demyelinating process in the LPC model at 7 dpi, while it did promote the maturation of OPCs together with remyelination at 14 dpi. We also found that the numbers of astrocytes and microglia were decreased after SA treatment in the LPC model; however, since these two types of cells play dual roles in the process of remyelination [
37], it is still not clear whether they are supportive or destructive.
Both the Ras/Raf/Mek/Erk and the PI3 K/Akt/mTOR pathways play important roles in OL lineage progression [
23‐
25]. Previous studies have shown that SA can suppress pain and pro-inflammatory factors by inhibiting the phosphorylation of Erk1/2 and p38 [
12]. Besides, the Erk1/2 pathway is associated with the survival, proliferation, migration, and differentiation of OPCs and myelination [
26,
38]. However, in our study, an inhibitor of MEK, an upstream kinase of Erk, did not block the SA-induced differentiation-promoting effects on OPCs, suggesting that these effects are not associated with the Erk1/2 pathway. Several studies have shown that mTOR, a downstream effector of AKT signaling, is crucial for OPC differentiation and myelination [
23,
39,
40]. Rapamycin, an mTOR inhibitor, can repress the differentiation of OPCs as well as the expression of most myelin proteins [
26]. Consistently, our experimental results suggested that SA increased the level of phosphorylated mTOR, which could be blocked by rapamycin. And the MBP
+ OL up-regulation by SA was shown to be antagonized by rapamycin. We also verified that a PI3 K inhibitor lowered the level of phosphorylated mTOR to the blank control level. Interestingly, in our experiments either U0126 or rapamycin alone repressed the maturation of OPCs, but SA plus U0126 did not significantly inhibit the maturation process. A possible explanation for this is that both the Akt/mTOR and Mek/mTOR pathways activate mTORC1 by interacting with the TSC1/TSC2 protein complex [
41‐
43], so SA may activate mTOR and induce OPC differentiation
via Akt when MEK is blocked by its inhibitor U0126. In the present study, we also found that SA promoted mTOR phosphorylation through the PI3 K pathway, which is in accord with previous research showing that SA activates the PI3 K/Akt pathway in hepatocytes [
44]. Thus, the induction of OPC differentiation by SA may mainly be mediated by the PI3 K/Akt/mTOR pathway.
In summary, we found for the first time that SA specifically promoted the differentiation and maturation of OPCs via the PI3 K/Akt/mTOR signaling pathway, alleviated the severity of EAE, and accelerated remyelination in the LPC model, suggesting the therapeutic potential of SA for demyelinating diseases.