Conditional Deletion of Foxg1 Alleviates Demyelination and Facilitates Remyelination via the Wnt Signaling Pathway in Cuprizone-Induced Demyelinated Mice

The massive loss of oligodendrocytes caused by various pathological factors is a basic feature of many demyelinating diseases of the central nervous system (CNS). Based on a variety of studies, it is now well established that impairment of oligodendrocyte precursor cells (OPCs) to differentiate and remyelinate axons is a vital event in the failed treatment of demyelinating diseases. Recent evidence suggests that Foxg1 is essential for the proliferation of certain precursors and inhibits premature neurogenesis during brain development. To date, very little attention has been paid to the role of Foxg1 in the proliferation and differentiation of OPCs in demyelinating diseases of the CNS. Here, for the first time, we examined the effects of Foxg1 on demyelination and remyelination in the brain using a cuprizone (CPZ)-induced mouse model. In this work, 7-week-old Foxg1 conditional knockout and wild-type (WT) mice were fed a diet containing 0.2% CPZ w/w for 5 weeks, after which CPZ was withdrawn to enable remyelination. Our results demonstrated that, compared with WT mice, Foxg1-knockout mice exhibited not only alleviated demyelination but also accelerated remyelination of the demyelinated corpus callosum. Furthermore, we found that Foxg1 knockout decreased the proliferation of OPCs and accelerated their differentiation into mature oligodendrocytes both in vivo and in vitro. Wnt signaling plays a critical role in development and in a variety of diseases. GSK-3β, a key regulatory kinase in the Wnt pathway, regulates the ability of β-catenin to enter nuclei, where it activates the expression of Wnt target genes. We then used SB216763, a selective inhibitor of GSK-3β activity, to further demonstrate the regulatory mechanism by which Foxg1 affects OPCs in vitro. The results showed that SB216763 clearly inhibited the expression of GSK-3β, which abolished the effect of the proliferation and differentiation of OPCs caused by the knockdown of Foxg1. These results suggest that Foxg1 is involved in the proliferation and differentiation of OPCs through the Wnt signaling pathway. The present experimental results are some of the first to suggest that Foxg1 is a new therapeutic target for the treatment of demyelinating diseases of the CNS.


Introduction
In the central nervous system (CNS), oligodendrocytes (OLs) are myelin-forming glial cells that play vital roles in rapid impulse conduction and normal axonal functions. Current studies have demonstrated that inflammatory stimuli or immune attacks can damage the myelin sheath, leading to OL death and myelin sheath loss, such as that observed in multiple sclerosis (MS), the most common demyelinating disease [1]. It has been reported that in early MS lesions, neural stem cells (NSCs) rooted in the region of the lateral ventricle-subventricular zone migrate, proliferate, and differentiate into oligodendrocyte progenitor cells (OPCs) induced by the injury signal of the myelin sheath and later differentiate to myelinating OLs to repair the damaged myelin [2]. However, OPCs are slow-cycling cells, and only long-term nutritional factors can stimulate their rapid proliferation and differentiation [3]. Furthermore, the repair ability of endogenous remyelination is limited, resulting in difficulties in the regeneration/repair of the myelin sheath in demyelinating diseases. Therefore, elucidating the regulatory mechanism of the correct differentiation of OPCs is crucial for understanding the myelination and remyelination processes in the CNS and is also fundamental to the treatment of demyelinating diseases [4]. Foxg1, also referred to as brain factor-1, is an important member of the Forkhead box transcription factor family, which plays dual roles in transcriptional activation and transcriptional repression [5]. Foxg1 is widely expressed in the cerebral cortex and is critical to the development of the CNS [6]. One or two homologous chromosome Foxg1 gene translocations, deletions, or mutations are closely related to various diseases associated with the occurrence and development of the CNS [7,8]. Previous studies have shown that loss of function or downregulation of Foxg1 reduces the proliferation of neural precursor cells, accompanied by early differentiation into neurons [9,10]. In addition, Tian et al. found that Foxg1 deletion increases the numbers of neurons and astrocytes at an early stage after birth in conditional Foxg1 gene-knockout mice, and they speculated that Foxg1 might inhibit neurogenesis and glial cell formation in the early stage after birth [11]. However, the regulation of Foxg1 in the development and differentiation of OPCs is still uncertain.
The Wnt signaling pathway plays an important role in the development and myelination of OPCs [12,13]. GSK-3b, a key kinase in the Wnt signaling pathway, negatively regulates the entry of catenin and then affects the expression of Wnt target genes [14]. Recent studies have demonstrated that GSK-3b activation promotes OPC differentiation, which may be mediated by the accumulation of nuclear b-catenin [15]. Nevertheless, whether the effect of Foxg1 on the development and maturation of OPCs is associated with the Wnt signaling pathway has not been reported.
To investigate the role of Foxg1 in the proliferation and differentiation of oligodendrocyte lineage cells and myelin regeneration, we conditionally knocked out Foxg1 in vivo to assess the loss and repair of myelin during demyelinating injury in mice, and we further explored its regulatory mechanism in vitro. Our findings revealed a previously-unknown function of Foxg1 in oligodendrocyte lineage cells, suggesting that downregulating the expression of Foxg1 in the treatment of demyelinating CNS diseases may alleviate demyelination and promote remyelination, thus providing a new gene therapy target for demyelinating CNS diseases such as MS.

Animals
Foxg1 cKO mice (1 male Nestin-CreER TM ; Foxg1 fl/fl mouse; 2 female Foxg1 fl/fl mice) were donated by Professor Chunjie Zhao from the Medical School of Southeast University. Wild-type ICR mice were purchased from the Experimental Animal Center of Xuzhou Medical University. All mice were housed with free access to food and water under a 12/12-h dark/light cycle and specific pathogen-free conditions. For Foxg1 conditional disruption in neural stem/progenitor cells (NSPCs), Nestin-CreER TM mice were crossed with Foxg1 fl/fl mice and induced with tamoxifen (TM; Sigma-Aldrich, St. Louis, MO, USA). The genotypes of all mice were determined by PCR analysis of tail genomic DNA with appropriate primers. Male and female mice were used for all experiments without bias. All experiments were performed according to the guidelines approved by Xuzhou Medical University Experimental Animal Ethics Committee.
The TM was dissolved in corn oil to a concentration of 10 mg/mL by shaking the solution for 3 h at 37°C. For CreER TM -mediated recombination, TM was intraperitoneally injected into mice at 1 mg/20 g body weight [16,17] 3 times on alternate days.

Experimental Model
Experimental demyelination was induced by feeding 7-week-old male mice 0.2% (w/w) cuprizone (CPZ, Sigma Aldrich, St. Louis, MO, USA) mixed into ground standard rodent chow [18,19]. The main ingredients in the normal diet for mice in this experiment were crude protein (C180 g/kg), crude fat (C40 g/kg), and crude fiber (B 50 g/kg). These mice were fed CPZ for 5 weeks and then allowed to remyelinate for 2 weeks with normal food.

Experimental Groups
Depending on the experimental purpose, mice were sacrificed at different times as follows: (1) to assess the knockout efficiency of Foxg1, 8 wild-type mice (WT group) and 8 Foxg1 cKO mice (cKO group) were sacrificed on day 7 after TM injection; (2) at the end of 5 weeks of CPZ administration, 32 mice in 4 groups (WT, WT?CPZ, cKO, and cKO?CPZ; 8 mice per group) were sacrificed to explore the effects of Foxg1 on CPZ-induced demyelination and OPC differentiation; (3) at the end of 4 weeks of CPZ administration, 24 mice in 3 groups (WT, WT?CPZ and cKO?CPZ; 8 mice per group) were sacrificed to explore the effects of Foxg1 on OPC proliferation; and (4) another 24 mice from the same groups (8 mice per group) were sacrificed to investigate the effects of Foxg1 on remyelination after 5 weeks of CPZ administration and another 2 weeks of recovery with normal chow. All mice received the same amount of chow each day.
In the OPC proliferation study, the mice were intraperitoneally injected with 5-bromo-2'-deoxyuridine (BrdU, Sigma-Aldrich, St. Louis, MO, USA) (50 mg/kg, 10 mg/ mL dissolved in normal saline) twice a day for 7 consecutive days from week 3 to week 4, and then sacrificed (Fig. 3A). To assess OPC differentiation, mice were fed a CPZ-containing diet for 1 week after BrdU administration for 7 consecutive days (Fig. 4A).

Morris Water Maze
The Morris water maze test (MWM) was used to evaluate spatial location learning and memory as described in previous studies [20,21]. All data were recorded using a computerized video system (EthoVision 3.1, Noldus Instruments, Wageningen, Gelderland, the Netherlands).

Histology and Immunofluorescence
Luxol fast blue staining and degrees of demyelination in three non-serial sections from each mouse were assessed semi-quantitatively in a blinded manner, as described previously [22]. The demyelination was scored as follows: 0, none; 1, rare foci; 2, a few areas; and 3, large (confluent) areas of demyelination.
For immunofluorescence, the brain sections were blocked with 5% bovine serum albumin (BSA) and 0.3% Triton X-100 (KeyGen Biotech, Nanjing, Jiangsu, China) in 0.01 mol/L phosphate-buffered saline (PBS) for 30 min at 37°C, followed by incubation with primary antibodies overnight at 4°C. The primary antibodies used were anti-CNPase were mounted with anti-fade mounting medium. The slides for BrdU staining were pretreated with solution containing 50% formamide, 280 mM NaCl, and 30 mM sodium citrate at 65°C for 2 h, incubated with 2 M HCl at 37°C for 30 min, and rinsed with 0.1 mol/L boric acid (pH 8.5) at room temperature for 10 min [2].

Image Acquisition and Quantification
Fluorescent images were captured using a confocal laser scanning microscope (Olympus FV10i, Tokyo, Japan) with appropriate excitation wavelengths. The digital images were measured using Image-Pro Plus 6.0 software (Media Cybernetics, Rockville, MD, USA). In the statistical analysis, at least 6 representative fields from randomlyselected images were acquired from each sample by a blinded observer, and then the average cell count/integrated optical density values were calculated [23]. To measure the proportion of OPCs in different differentiation stages in vitro, each dish was scanned with a 20 9 objective lens in 600 lm 9 450 lm format in the x-y direction. The number of NG2/GFP, O4/GFP or CNPase/ GFP double-positive cells among GFP-positive cells in each field was counted by a blinded observer [2].

Primary Culture of Rat OPCs
The rat OPC proliferation culture was maintained as previously described [24,25]. Isolated OPCs were plated at 10,000 cells/cm 2 on poly-L-lysine-coated flasks and cultured in DMEM/F12 medium supplemented with 2% B27, 10 ng/mL platelet-derived growth factor AA (PDGF-AA, Gibco, Grand Island, NY, USA), and 10 g/mL basic fibroblast growth factor (bFGF, Gibco) for 3 days; then, the medium was replaced with DMEM/F12 medium without PDGF-AA and bFGF for 1 day to generate preOLs. For oligodendrocyte differentiation, 10% fetal bovine serum (FBS) was added to the preOL medium and cultured for 7 days. The medium was changed every 2 days.

Quantitative Real-Time Polymerase Chain Reaction (qRT-PCR)
Genomic RNA was extracted with TRIzol reagent (Invitrogen, Carlsbad, CA, USA) according to the manufacturer's instructions and as previously described [26]. The sense and antisense primers for GSK-3b were as follows: forward: 5 0 -TCCCTCAAATTAAGGCACATC-3 0 and reverse: 5 0 -CACGGTCTCCAGTATTAGCATC-3 0 . The expression level of 18S ribosomal RNA (rRNA) served as an internal control for the samples, and was assessed using the following sense and antisense primers: forward: 5 0 -CCTGGATACCGCAGCTAGG A-3 0 and reverse: 5 0 -GCGGCGCAATACGAATGCCCC-3 0 . The relative level of Foxg1 mRNA expression was calculated according to the standard 2 -DDCt method by normalization to the 18S rRNA mRNA level.

Lentiviral Vector Production
A lentivirus encoding small hairpin RNA (shRNA) for Foxg1 was designed and synthesized by GeneChem Co., Ltd (Shanghai, China). The Foxg1 locus on chromosome 2 and its 200-bp flanking sequences were amplified by PCR from genomic rat DNA and inserted into the GV248 vector (the functional element is Ubi-EGFP-MCS-IRES-puromy-cin). The shRNA sequence for Foxg1 was 5 0 -TCGGGCCAAGCTAGCCTTTAA-3 0 . To generate the construct, the scrambled sequence 5 0 -TTCTCCGAACGTGTCACGT-3 0 was inserted. In the scrambled sequence, the nucleotides were randomly added with no target sequence tracks.

EdU Labeling of OPCs
For EdU labeling, 3.5910 4 cells were seeded into each well of a 48-well plate in DMEM/F-12 medium (1:1) supplemented with 10% FBS. Twenty-four hours later, EdU (RiboBio, Guangzhou, China) was added to the medium at 10 lmol/L. Another 24 h later, the cells were fixed with 4% paraformaldehyde for 30 min. For EdU staining, the cells were then incubated with freshly-made 19 Apollo Ò 567 reaction cocktail for 30 min at room temperature in the dark. Then, the cells were incubated in 0.5% Triton X-100 in PBS for 10 min at room temperature. After washing twice with PBS, the cells were fixed in methanol and then stained with Hoechst 33342. The percentage of EdU-positive cells was calculated as the number of Apollo Ò 567-stained cells/the number of Hoechst 33342-stained cells.

Statistical Analysis
Data were analyzed with SPSS software version 19.0 (IBM, Armonk, NY, USA) and are expressed as the mean ± SEM. T-tests or one-way analysis of variance (ANOVA) followed by the Newman-Keuls or Tukey's HSD post tests were used for comparisons between two or multiple groups, respectively. Statistical significance was set at P \ 0.05.

Conditional Ablation of Foxg1 Ameliorates Behavioral Deficits and Demyelination Induced by CPZ
On the first day (day 0) of CPZ treatment, the mice were intraperitoneally injected with TM to induce Foxg1 gene b Fig. 1 Foxg1 cKO relieves CPZ-induced learning and memory impairments in mice. A Schematic of the cuprizone (CPZ) and tamoxifen (TM) administration time points during experiment. Adult 7-week-old mice were fed a diet containing 0.2% CPZ for 5 weeks (demyelination phase); TM was intraperitoneally injected (3 times, 24 h apart) from day 0 after feeding the CPZ diet; mice were sacrificed immediately after the knockout (Fig. 1A). The results showed that, compared with control littermates, Foxg1 expression on neural stem cells in the subventricular zone (Fig. 1C, D) or OPCs in the corpus callosum region (Fig. 1E, F) was significantly reduced in Foxg1-cKO mice on day 7 after TM injection. Studies have shown that CPZ administration results in a decline in learning and memory in mice [29,30]. The MWM test showed that Foxg1 cKO significantly shortened the prolonged mean latency from day 2 to day 4 (Fig. 1G,  H), and it significantly decreased the latency to the platform on day 5 (Fig. 1G, I). The crossing number of Foxg1-cKO mice was clearly increased compared with the WT?CPZ mice (Fig. 1J). These results suggested that Foxg1 cKO significantly alleviates the learning and memory impairments induced by CPZ in mice. LFB staining showed that myelin was intact in the corpus callosum of WT mice, but it had almost entirely disappeared in the WT?CPZ mice ( Fig. 2A). The demyelination score was significantly lower in the Foxg1 cKO?CPZ group than in the WT?CPZ group (Fig. 2D). The statistical data from the myelin basic protein (MBP) immunofluorescence staining was consistent with the LFB staining results (Fig. 2B, E). These results indicated that demyelination induced by CPZ is significantly relieved by the absence of Foxg1.

Foxg1 cKO Decreases Proliferation but Promotes the Differentiation of OPCs in CPZ-Induced Demyelination
BrdU labeling was used to assess cell proliferation (Fig. 3A) and differentiation (Fig. 4A) in the corpus callosum, and the results showed that the number of BrdU-positive cells was significantly lower in the Foxg1 cKO?CPZ group than the WT?CPZ group (Fig. 3C, D). Furthermore, the increase in percentage of NG2 ? cells (Fig. 3E, F) and O4 ? cells (Fig. 3J) cells in the WT?CPZ group was prevented by Foxg1-cKO treatment. The number of proliferating OPCs, indicated by NG2 ? /BrdU ? (Fig. 3G, H) or BrdU ? /O4 ? (Fig. 3I, K), was also decreased; however, the number of new mature oligodendrocytes labeled with BrdU ? /MBP ? (Fig. 4C, D), BrdU ? / CNPase ? (Fig. 4E, F), and BrdU ? /MAG ? (Fig. 4G, H) differentiated from the OPCs was significantly higher in the Foxg1 cKO?CPZ group than in the WT?CPZ group. These data suggested that Foxg1 cKO decreases the production or proliferation of OPCs but promotes their differentiation.

Foxg1 cKO Facilitates Myelination and the Recovery of Cognitive Function During Remyelination
To study the role of Foxg1 in the regeneration of OLs after CPZ-induced myelin sheath injury, TM was administered on day 1 of CPZ withdrawal (Fig. 5A). Behavioral results showed that the average latency was significantly longer in the WT?CPZ than the WT group; however, Foxg1 deletion in CPZ-treated mice clearly decreased the latency (Fig. 5B, C). In the spatial exploration experiment on day 5, the number of platform crossings was significantly higher in the Foxg1 cKO?CPZ than the WT?CPZ group (Fig. 5D). These results suggested that Foxg1 cKO significantly promotes the recovery of learning and memory after CPZ withdrawal in mice.
After 2 weeks of feeding without CPZ, the demyelination score was decreased (Fig. 5F, G) and the fluorescence intensity of MBP significantly enhanced (Fig. 5H, I) in the Foxg1-cKO mice. These results indicated that Foxg1 deficiency favors myelin repair after CPZ-induced demyelinating injury.

Foxg1 cKO Inhibits Proliferation but Promotes the Differentiation of OPCs In Vitro
In vitro, GFP-tagged shRNA knockdown of Foxg1 using lentiviral transfection was required to confirm its function in the proliferation and differentiation of cultured OPCs. The results of immunofluorescence staining (Fig. 6A, B) and Western blotting (Fig. 6D) demonstrated that Foxg1 knockdown strongly decreased the expression of Foxg1 in primary cultured rat OPCs. The lentiviral transfection efficiency was defined by GFP fluorescence (Fig. 6C). The results of EdU staining showed that the number of EdU ? cells was significantly smaller in the Foxg1 shRNA than the control group (Fig. 6E, F). These results indicated that, to a certain extent, knockdown of Foxg1 decreases the proliferation of OPCs in vitro, suggesting that Foxg1 participates in the regulation of OPC proliferation.
To confirm whether Foxg1 regulates OPC differentiation, we downregulated the level of Foxg1 in OPCs and analyzed the number of immature and mature OLs. In contrast to the control group, most of the cells in the shRNA group were labeled with CNPase (Fig. 6I), and only a few were labeled with NG2 (Fig. 6G) or O4 (Fig. 6H). The number of O4-positive cells was significantly lower and CNPase-positive cells significantly higher in the Foxg1 shRNA than in the Ctrl group (Fig. 6J), suggesting that Foxg1 plays a negative regulatory role during OPC differentiation into OLs.

Foxg1 May Participate in the Proliferation and Differentiation of OPCs Through the Wnt Signaling Pathway
To explore whether Foxg1 influences Wnt signal activation, we assessed the expression of GSK-3b and b-catenin. The results showed that the level of GSK-3b mRNA (Fig. 7A) and protein (Fig. 7B) was significantly higher in the Foxg1 shRNA than in the control group, while the expression of b-catenin was significantly decreased in Foxg1-knockdown OPCs (Fig. 7C). The GSK-3b inhibitor SB216763 reversed the decrease in b-catenin induced by Foxg1 knockdown (Fig. 7C). Moreover, SB216763 treatment also clearly increased the number of EdU ? cells (Fig. 7D, E) and the proportions of NG2 ? (Fig. 7F, I) and O4 ? cells (Fig. 7G, I) and decreased the proportion of CNPase (Fig. 7H, I) when compared with the Foxg1 shRNA group. These results indicated that Foxg1 might be involved in the proliferation and differentiation of OPCs through the Wnt signaling pathway. b Fig. 3 Conditional knockout of Foxg1 decreases the proliferation of oligodendrocyte precursor cells in the corpus callosum (CC) of mice induced with cuprizone (CPZ). A Schematic of CPZ and BrdU administration time points during the experiment. Adult 7-week-old mice were fed a diet containing 0.2% CPZ for 4 weeks (demyelination phase) to assess the proliferation of intrinsic OPCs; Tamoxifen (TM) was intraperitoneally injected (3 times, 24 h apart) from day 0 after starting the CPZ diet; BrdU was intraperitoneally injected twice a day for 7 consecutive days, and then the mice were sacrificed.

Discussion
As described in previous reports, Foxg1 is abundantly expressed in the CNS [31] and plays pivotal roles in organogenesis through the regulation of proliferation and the specification of cell fate [32]. However, the role of Foxg1 in the oligodendroglial lineage and the underlying mechanisms remain unclear. Therefore, the present study was designed to determine the effect of Foxg1 and the mechanisms underlying the regulation of the Wnt signaling pathway following CPZ-induced demyelination. CPZ is a copper chelator that impacts cell metabolism and leads to oligodendrocyte death and demyelination accompanied by weight loss and behavioral disorders [33]. The CPZ-fed C57BL/6 mouse model has been increasingly used to study demyelination and remyelination in the CNS [33,34]. The present results are consistent with previous reports [35,36], demonstrating that we successfully replicated the CPZ-induced demyelination model in the ICR strain of mice [37]. However, for the first time, we found that conditional knockout of Foxg1 in NSPCs reversed the demyelination and spatial learning and memory impairments; moreover, a more evident remyelination was found after CPZ withdrawal. It has been reported that different subcellular localizations of Foxg1 control the machinery that causes cell differentiation, replication, and bioenergetics. A fraction of Foxg1 is recruited to mitochondria and plays a major role in neuronal survival, differentiation, and plasticity [38]. In addition, dietary triheptanoin rescues oligodendrocyte loss in a mouse model of Canavan disease [39], as well as the functional and molecular abnormalities in Foxg1 ?/mice [40]. Thus, it should be noted that the food used in our study was a normal diet. To induce demyelination, 0.2% (w/w) CPZ was mixed into ground standard rodent chow. In addition, each group of mice received the same amount of chow. Thus, we confirmed that Foxg1 might participate in the repair of myelin sheath damage in mice with CPZinduced demyelination.
Oligodendrocytes are derived from OPCs [41], which populate the CNS starting from embryonic development [42,43]. Previous studies [44,45] have demonstrated that demyelinating injury induces OPC proliferation; however, studies on the differentiation of OPCs into mature oligodendrocytes and remyelination are limited. The mechanisms underlying the effect of Foxg1 on the regulation of demyelination and remyelination remain to be clarified. Here, we found that CPZ administration increased the number of OPCs, which indicated that CPZ injury initiates the endogenous repair process and promotes the production of OPCs from neural stem cells of the subventricular zone region and migration to the injured area [46]. In the CPZinduced demyelinated mouse corpus callosum, OPC proliferation was decreased by Foxg1 cKO. Moreover, double labeling using BrdU and cell-specific markers showed that Foxg1 cKO promoted OPC differentiation into mature OLs. Previous research has demonstrated that Foxg1 may be necessary for maintenance of the NSC pool in the CNS and that genetic inactivity of Foxg1 promotes both gliogenesis and neurogenesis [11]. NSCs are maintained in a quiescent state in the adult CNS [47]. Although it has been reported that Foxg1 cKO in nestin-positive NSCs promotes neurogenesis and gliogenesis [11], it did not markedly change the myelin sheath and behavior in mice fed a normal diet in our study. We conclude that the change was so mild that there was no marked qualitative difference between the groups. However, the CPZ diet induced very serious demyelination accompanied by a change in the stem cell niche and OPC proliferation, and under this pathological situation, Foxg1 cKO clearly promoted OPC differentiation. In vitro, purified primary OPCs were used to assess the effects of Foxg1 inhibition on OPC proliferation and differentiation. It has been demonstrated that the loss of Foxg1 leads to cycle exit and promotes the differentiation of premature cells [48,49]. Consistent with previous reports [9][10][11], Foxg1 knockdown inhibited the proliferation and promoted the differentiation of OPCs under normal culture conditions. As a result, the number of OPCs in the CPZ-treated corpus callosum area was reduced due to accelerated differentiation. The differentiated mature OLs encapsulated the axons of the neurons to form new myelin sheaths, thereby alleviating the myelin damage caused by CPZ or accelerating remyelination.
The Wnt/b-catenin signaling pathway plays an important role in regulating cell proliferation and differentiation [50][51][52]. Studies have shown that inhibition of GSK-3b expression in the Wnt signaling pathway inhibits the differentiation of OPCs while promoting their proliferation [53,54]. Here, we found a significant increase in GSK-3b at the mRNA and protein levels in OPCs after Foxg1 knockdown. We used 10 lmol/L SB216763 to inhibit the function of GSK-3b [55,56], and found that this treatment b Fig. 7  reversed the effect of Foxg1 on OPC proliferation and differentiation and the nuclear level of b-catenin. These results are in agreement with reports in the literature [15]. Together with the results of the in vivo experiments performed here, it can be concluded that conditional knockout or knockdown of Foxg1 effectively facilitates the differentiation of OPCs into OLs and promote the recovery of damaged myelin, and the Wnt/b-catenin signaling pathway is involved in this process. Given the increasing importance of glia-glia crosstalk and the inflammatory microenvironment in demyelination or remyelination [57][58][59], future studies are needed to focus on the microglia, astrocytes, and even the interaction between microglia, astrocytes, and oligodendrocytes, to further clarify the role of the Wnt/b-catenin signaling pathway in CPZ-induced demyelination or remyelination.
In summary, the present study provides evidence that, in CPZ-induced demyelinating mice, Foxg1 knockout inhibits the proliferation but promotes the differentiation of OPCs into mature OLs by regulating the activity of the Wnt/bcatenin signaling pathway, which ultimately reduces the severity of demyelination and promotes remyelination. Therefore, Foxg1 might be a promising novel target to enhance endogenous remyelination in patients with demyelinating diseases such as MS. Further experiments are required to investigate the precise targets of Foxg1 in the Wnt/b-catenin signaling pathway and its interactions with other types of glial cells involved in demyelinating diseases in the CNS.

Conflict of interest
The authors have no conflicts of interest to declare.
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