GFAP expression is regulated by Pax3 in brain glioma stem cells
- Authors:
- Published online on: July 7, 2016 https://doi.org/10.3892/or.2016.4917
- Pages: 1277-1284
Abstract
Introduction
Malignant gliomas are the most common type of primary brain tumors (1), of which patients have a notably high likelihood of relapse after treatment (2–4). Glioblastomas are understood to evolve from brain glioma stem cells (BGSCs). BGSCs have the capabilities of self-renewal, and may render themselves profitable to the survival of tumors by conferring resistance to therapeutic treatments (5,6). It was initially proposed that acute myelogenous leukemia may evolve from a subset of precursor stem cells, and considerable efforts have been devoted to studying this sub-population of cells in numerous cancers since (7). Stem cells, for example, exhibit many of the hallmarks inherent to malignant tumors, including the abilities to proliferate, invade and metastasize (5).
Stem cells expressing the CD133 membrane protein are markedly pronounced within cells of malignant gliomas (7,8). Furthermore, the encephalic inoculation of CD133+ stem cells into NOD-SCID mice results in tumor growth (9). Thus, CD133+ stem cells are likely to be important for tumor recurrence. Paired box 3 protein (Pax3) is a member of the paired box (Pax) family of transcription factors that is normally expressed during embryonic development, but has recently been implicated in tumorigenesis (8). The expression of Pax3, for example, was found to be positively correlated with melanoma progression (10–12). In addition, GFAP is a major intermediate filament protein, where it likely plays a critical role in mature astrocytes owing to its high abundance and strong conservation among vertebrates. Pax3 has previously been reported to negatively regulate the expression of GFAP during the differentiation of astrocytes from neural stem cells (NSCs) (13,14). In addition, Pax3 overexpression can be detected during the process of the astrocyte precursor cell proliferation and can maintain the high malignancy in gliomas by negatively regulating GFAP expression in glioma cells (15). Thus, we speculated that GFAP is a Pax3-responsive gene in BGSCs. In these studies, we attempted to examine the expression of Pax3 and to determine whether Pax3 could bind to the element of the GFAP promoter in BGSCs.
Materials and methods
Cell lines and reagents
Human BGSCs were kindly gifted by Soochow University, China. Human malignant glioma cell line (U87MG) and normal human astrocytes (1800) were obtained from the Cell Library of the Chinese Academy of Sciences (Shanghai, China). BGSCs were cultured at 37°C in 5% CO2 in a 1:1 mix of Dulbecco's modified Eagle's medium and Ham's F-12 medium (DMEM/F-12) (Gibco, Grand Island, NY, USA) containing 10 ml B27, 10 µg EGF, 10 µg FGF, 5 ml L-glutamine, 5 ml MEM-vitamin solution, 5 ml sodium pyruvate, 5 ml MEM non-essential amino acids (Gibco), and 5 ml penicillin-streptomycin solution (HyClone, Logan City, UT, USA). U87MG cells were cultured at 37°C in 5% CO2 in DMEM supplemented with 10% fetal bovine serum (FBS), 2 mM L-glutamine and 100 U/ml penicillin-streptomycin (Gibco). The normal astroctyes (1800) were cultured at 37°C and 5% CO2 in modified RPMI-1640 medium (HyClone) supplemented with 10% FBS, 2 mM L-glutamine and 100 U/ml penicillin-streptomycin (Gibco). Culture medium was altered every 3–4 days. U87MG and 1800 cells were split using 0.25% trypsin. BGSCs were split using StemPro Accutase. The present study obtained ethical approval from the Affiliated Hospital of Nantong University, China [approval ID: (2013)040].
RT-PCR
Total RNA was extracted from cells with TRIzol (Invitrogen, Carlsbad, CA, USA), from which cDNA was reverse transcribed using the Omniscript RT kit (Qiagen) aaccording to the manufacturer's instructions. The sequences for primers used were as follows: H-Pax3-F, 5′-AAGCCCA AGCAGGTGACAA-3′ and H-Pax3-R, 5′-ATGGAACTCACTGACGGCAC-3′; H-GFAP-F, 5′-AGATCCGCACGCAGTA TGA-3′ and H-GFAP-R, 5′-AGTCGTTGGCTTCGTGCTT-3′; H-β-actin-F, 5′-CATGAAGTGTGACGTGGACATC-3′ and H-β-actin-R, 5′-GGACTCGTCATACTCCTGATTG-3′. The thermal cycles were: 95°C for 30 sec, 68°C for 30 sec, and 72°C for 30 sec for 35 cycles for β-actin, and 95°C for 30 sec, 58°C for 30 sec, and 72°C for 30 sec for 35 cycles for Pax3.
Western blotting
Expression levels of β-actin, Pax3 and GFAP proteins were determined via western blotting with specific antibodies as previously described (16). The following antibodies were used: primary antibodies against β-actin (1:2,000 dilution), Pax3 (1:500) and GFAP (1:1,000); all of which were obtained from Abcam (Cambridge, MA, USA).
Immunofluorescence microscopy
Dispersed BGSCs were smeared onto a Poly-L-lysine glass slide. Cells were washed with phosphate-buffered saline (PBS), fixed in 4% paraformaldehyde for 30 min, permeabilized in 0.1% Triton X-100 for 30 min, and blocked against non-specific binding in 5% BSA (Amresco, Solon, OH, USA) for 45 min at room temperature. Subsequently, cells were incubated with rabbit anti-Pax3 polyclonal (1:100), GFAP monoclonal (1:100) (both from Abcam), anti-human nestin (1:100; Alexa Fluor 488l eBioscience, San Diego, CA, USA), and anti-human CD133-APC antibodies (1:100; Miltenyi Biotec) overnight at 4°C. The slides were then washes 3 times with PBS, and incubated with Cy3 or FITC fluorescently-labeled secondary antibodies for 2 h at room temperature. DNA was stained by incubating the slides in 4′,6-diamidino-2-phenylindole (DAPI) (0.2 mg/ml) for 2 min immediately following incubation with secondary antibodies. Slides were stored at 4°C in the dark and visualized with a Leica fluorescence microscope (Germany). All assays were performed 3 times in duplicate.
siRNA transfection
Pax3 was knocked down as previously described (15), using siRNA sequences purchased from Biomics (Jiangsu, China). The siRNA sequences were: Pax3 sense, 5′-CGCAUCCUGAGAAGUAAAUdTdT-3′ and Pax3 antisense, 5′-AUUUACUUCUCAGGAUGCGdTdT-3′; negative control (NC) sense, 5′-UUCUCCGAACGUGUCACGUTT-3′ and NC antisense, 5′-ACGUGACACGUUCGGAGAATT-3′. siRNAs were transfected into BGSCs in 6-well plates (1 mg/ml) using the MicroPoly-Transfecter Cell Reagent (Invitrogen) completed according to the manufacturer's instructions.
Transient transfections and differentiation
Plasmid vectors for overexpressing Pax3 were constructed by GeneChem (Shanghai, China). Transient transfections were carried out using the MicroPoly-Transfecter Cell Reagent according to the manufacturer's instructions. To induce differentiation, the transfected BGSCs were seeded onto coverslips coated with poly-L-lysine within 24-well plates, and cultured in DMEM/F-12 supplemented with 1% FBS for 3 days. Next, the neurospheres were fixed and processed for immunofluorescence microscopy as previously described. A subset of cells were omitted from immunofluorescence microscopy, and were incubated at 37°C for 24 h after transfection.
CCK-8 cell proliferation assay
Cells at 12 h post-transfection were seeded into 96-well plates at a density of 4,000 cells/well. Next, cell viability was determined using the Cell Counting Kit-8 (CCK-8; Dojindo, Shanghai, China). Briefly, 100 µl DMEM/F-12 and 10 µl CCK-8 reagent were added to each pre-cultured film, whereupon the plates were incubated for 1.5 h at 37°C. The absorbance was determined at a wavelength of 450 nm using a Multiskan MK33 microplate reader (Thermo Electron Corporation, Shanghai, China).
Cell invasion assay
A cell invasion assay was performed using 24-well tissue culture plates (BD Biosciences, Bedford, MA, USA) consisting of an 8-µm polyethylene terephthalate membrane coated with a Matrigel basement membrane matrix (100 µg/cm2). In brief, the Matrigel (R&D Systems, Minneapolis, MN, USA) was rehydrated overnight at 4°C. The Transwell membranes were pre-coated with 24 mg/ml Matrigel. Two days after transfection, the cells (5×104) were seeded into the upper chamber with DMEM/F-12, and the lower chamber was filled with DMEM containing 10 ml B27, 10 µg EGF, 10 µg FGF, 5 ml L-glutamine, 5 ml MEM-vitamin-solution, 5 ml sodium pyruvate, 5 ml MEM non-essential amino acids, and 5 ml penicillin-streptomycin solution as a chemoattractant. The invasion assay was carried out in a 5% CO2 humidified chamber at 37°C for 48 h, and cells on the upper surface of the filters were removed by wiping the upper surface of the membrane with a cotton swab. The filter membrane was fixed in 4% paraformaldehyde, and stained with Coomassie blue. The degree of invasion was quantified by counting the cells that migrated to the lower side of the filter in at least six random fields at a magnification of ×100 using a fluorescence microscope. Experiments were repeated 3 times in triplicate.
Apoptosis detection
Cells were trypsinized, counted, washed twice with ice-cold PBS, and resuspended in 1X binding buffer (pH 7.4) containing 10 mM HEPES/NaOH, 140 mM NaCl, and 2.5 mM CaCl2. Next, 100 µl cell suspension was stained with 5 µl Annexin V-FITC fluorescent label (R&D Systems Europe Ltd., Abingdon, UK) and 10 µl propidium iodide (PI) (Sigma) for 15 min at room temperature in the dark. Finally, 400 µl of binding buffer was added to each sample, which was immediately held on ice prior until analysis on a FACSCalibur flow cytometer (BD Pharmingen, San Diego, CA, USA), for which 105 cells/sample were analyzed.
Monoclonal formation
The original neural cells were digested with StemPro Accutase into single cell suspension. Next, the digests were diluted to 40 cells/ml with serum-free medium containing B27, bFGF and EGF, of which 50 µl of this cell suspension was inoculated/microwell of a 96-well plate. Cells were centrifuged at 1,000 × g, to which 3 parts supernatant was combined with 1 part fresh serum-free culture medium, and bFGF and EGF were added for a final concentration of 20 ng/ml. Next, 100 µl serum-free culture mixture was added to each microhole, whereupon cells were cultivated at 37°C and 5% CO2. Finally, the division and cloning of the single cells were observed with microscopy.
Chromatin immunoprecipitation
Chromatin was immuneprecipitated with a ChIP assay kit (Upstate Biotechnology, Lake Placid, NY, USA) completed as per the manufacturer's instructions. Briefly, BGSCs were lysed, where upon the chromatin was immunoprecipitated with anti-Pax3 polyclonal antibodies (sc-376215; Santa Cruz Biotechnology, Inc., Santa Cruz, CA, USA).
Luciferase reporter assay
The length promoter plasmid pGFAP1600 of the human GFAP gene was cloned into a pGL3-Basic luciferase reporter vector (Promega, Madison, WI, USA) and amplified via PCR. The oligonucleotide PCR primer sequences used to detect the fragment of the pGFAP were as follows: GFAP F (KpnI), 5′-CCCGGTACCAAGCAGAC CTGGCAGCATTG-3′ and GFAP R (HindIII), 5′-CGGAAGC TTGCCCGGGTGCCCCTGGCAAC-3′. Mutant-promoter constructs were created by deleting the nucleotides corresponding to the P1 and P2 probes (P1 F5, 5′-CATGCCCATGA CTCACCTTGGCACAG-3′ and R5, 5′-GTGAGTCATGGGCATGAAGAGGAGGC; P2 F7, 5′-GGGATTACGCCACCCCACTCAGCCCT-3′ and R7, 5′-GGGGTGGCGTAATCCCAGCACTTTGG-3′) of pGFAP1600, either individually or in combination, using a Pfu Turbo DNA polymerase from a QuikChange kit (Stratagene, La Jolla, CA, USA). The mutant-promoter constructs were termed pGFAP1600-DelP1 (deletion of 5 nucleotides within P1) or pGFAP1600-DelP2x (deletion of 8 nucleotides within P2). The human Pax3 was achieved by cloning the cDNA fragment into a pCI vector in HEK 293T cells. All constructs were confirmed by sequence validation. Normal or mutated GFAP promoter reporter plasmids were transfected together with the PRL (Promega) vector into HEK 293T cells using Lipofectamine 2000. HEK293T cells were used for luciferase assay since these cells are more easily transfected in comparison with BGSCs. Twenty-four hours after transfection, the cells were lysed and assayed using the Dual-Luciferase Assay kit (Promega). Promoter activity was measured by comparing luciferase levels.
Electrophoretic mobility shift assay
Putative interactions between Pax3 and GFAP mRNA transcripts were monitored via the electrophoretic mobility shift assay. Nuclear components of HEK 293T cells transfected with overexpression-Pax3 were extracted according to NE-PER Nuclear and Cytoplasmic Extraction Reagents (Pierce, Rockford, IL, USA) and electrophoretic mobility shift assays (EMSA) were exactly performed as previously described (17). First, we designed fluorescently-labeled normal and mutated probes. The sequence of the normal and mutated oligo nucleotides used in this experiment were: P1 probe Fw, 5′-ATGCCCAGTGAATGACTCAC-3′ and Rw, 5′-GTGAGTCATTCACTGGGCAT-3′; PIM probe Fm, 5′-ATGCCCACTGTATGACTCAC-3′ and Rm, 5′-GTGAGTCATACAGTGGGCAT-3′. For supershift experiments, nuclear extracts were pre-incubated with anti-Pax3 polyclonal antibodies (Abcam) before adding the labeled probes.
Statistical analysis
All statistical analyses, including the t-test was carried out using GraphPad Prism software (version 6; GraphPad Software, La Jolla, CA, USA).
Results
Identification of BGSCs and Pax3 and GFAP mRNA expression
We performed immunofluorescence staining with CD133+ and nestin antibodies to identify BGSCs. Through immunofluorescence, the nuclei of the supposed BGSCs were stained blue, the cytoplasm red, and the cell membrane stained green, therefore confirming the expression of CD133+ and nestin BGSC markers (Fig. 1A). We also determined whether Pax3 enhanced GFAP expression in the BGSCs using immunohistochemical staining (Fig. 1B), and observed that GFAP and Pax3 proteins co-localized in the cytoplasm of the BGSCs. Furthermore, we measured the expression of Pax3 and GFAP in the U87MG human glioma cell, BGSC and 1800 normal human astrocyte lines by RT-PCR. Pax3 was highly expressed in the BGSCs compared with that noted in the normal human astrocytes (Fig. 1C). In addition, we found that a single BGSC could form a colony of 50 BGSCs by proliferation, suggesting the observed colony formation resulted from the ability of BGSCs to self-renew and proliferate, rather than the recruitment of individual BGSCs (Fig. 1D).
Pax3 decreases the apoptosis, enhances the invasion and promotes the proliferation of BGSCs
The proportion of BGSCs undergoing apoptosis was determined using an Annexin V/PI apoptosis detection kit coupled to flow cytometry. We found that a significantly greater proportion of siPax3-transfected BGSCs underwent apoptosis relative to the control BGSCs (P<0.01), while the apoptotic index of BGSCs transfected to overexpress Pax3 was significantly lower than that of the untransfected cells (P<0.01; Fig. 2A). Subsequently, we performed a cell invasion assay to determine the influence of Pax3 on the invasion of BGSCs. The number of invading BGSCs transfected with a Pax3-knockdown siRNA was significantly lower (14±5) than that of the untransfected cells (78±12; P<0.01). Moreover, the number of BGSCs transfected with a Pax3-overexpression vector (152±6) was markedly greater than that of the normal control cells (P<0.01). The above results suggest that Pax3 enhances BGSC invasion in vivo (Fig. 2B).
We also determined the influence of Pax3 expression status on the proliferation of BGSCs using the CCK-8 assay. We found that the proliferation of siPax3-transfected BGSCs was significantly inhibited (P<0.05), but there was a significant increase in proliferation in the overexpression Pax3 plasmid-transfected BGSCs (P<0.05; Fig. 2C). These data suggest that Pax3 promotes the proliferation of BGSCs.
Pax3 binds the GFAP promoter
Pax3 is a transcription factor containing a paired domain that recognizes consensus sequences harboring a GTTCC motif and a paired-type homeodomain that binds with a consensus sequence harboring an ATTA motif (13). We used chromatin immunoprecipitation to determine whether Pax3 can bind to the promoter region of GFAP in the context of native chromatin. First, we analyzed the gene promoter sequences within 2.0 kb upstream of the transcriptional start site of genes using a pair of primers of 250–300 bp (GFAP F1, 5′-CCAGGTCCCCAGTTCATAGCA-3′ and GFAP R1, 5′-TCCTTCCACATCAGCCTCCC-3′; GFAP F2, 5′-TGTCCAAATGCAGAGCATACCC-3′ and GFAP R2, 5′-GGCGCAACCACGACTCACTG-3′; GFAP F3, 5′-AGGCTGAGGTGAGGGGATCA-3′ and GFAP R3, 5′-AATGCTGCCAGGTCTGCTTG-3′; GFAP F4, 5′-CAAGCAGACCTGGCAGCATT-3′ and GFAP R4, 5′-CTGAATAGAGCCTTGTTCTCCACC-3′; GFAP F5, 5′-CACCGGCGGTGGAGAACAAG-3′ and GFAP R5, 5′-TCTGGGGATGGATGGGTTTG-3′; GFAP F6, 5′-TCCCCAGAGGTTCTTCCCATC-3′ and GFAP R6, 5′-GTGGCAGTGGAGGTCCTGATAG-3′; GFAP F7, 5′-CAGGACCTCCACTGCCACATAGA-3′ and GFAP R7, 5′-TTTCATAACCCAGGCATTATCTCACT-3′; GFAP F8, 5′-AGTTGGAAAGCAGGTCAGAGGTCA-3′ and GFAP R8, 5′-GGAAGGTGGGTCAAGAAAGGGTT-3′; GFAP F9, 5′-ACCCTTTCTTGACCCACCTTCC-3′ and GFAP R9, 5′-TCTGGCTCTGCTCGCTCCTG-3′; GFAP F10, 5′-CCTCAGTGGGGTGAGGGGAGC-3′ and GFAP R10, 5′-GGGGCATTCGAGCCAGGGAG-3′). We also used an anti-Pax3 antibody specific for targeting an intron sequence of GFAP. The binding of Pax3 to the P1 and P2 regions was subsequently demonstrated by PCR performed with primers specific to BGSCs (Fig. 3A).
Subsequently, we referred to the study by Cao et al that described two Pax3 protein binding sites, designated P1 (5′-ATGCCAGTGAATGACTCAC-3′, spanning from −949 to −979 bp on the positive strand) and P2 (5′-GGGATTACAAGCATGAGCCACC-3′, spanning from −2,172 to −2,183 bp on the positive strand) (18). According to these results, we constructed two recombinant normal and mutated promoters of GFAP, and performed luciferase reporter gene assays to determine mRNA transcript expression. The normal pGFAP1600 luciferase promoter construct showed low transcription activity, while inducing overexpression of Pax3 resulted in a notable increase in transcriptional activity. Furthermore, the absence of P1 in the promoter region resulted in a notable decrease in transcription activity, whereas the absence of the P2 promoter region had no obvious suppression on transcription (Fig. 3B). Together, these results indicated that: i) Pax3 can regulate GFAP; and ii) that P1 is the binding region for transcription factors. Next, the EMSA revealed that Pax3 binds to the P5 promoter region of GFAP. The double-stranded oligonucleotides corresponding to the predicted cis-element of the GFAP promoter region formed sequence-specific DNA/protein complexes with the nuclear extracts of Pax3-expressing HEK293T cells, while the mutated P1 probes failed to generate such a DNA/protein complex during EMSA (Fig. 3C). Finally, we performed EMSA-supershift analysis using a fluorescently-labeled anti-Pax3 antibody to stain the nuclear extract of HEK 293T cells with overexpression of Pax3. The presence of the anti-Pax3 antibody generated the supershift band.
Pax3 inhibits GFAP expression in BGSCs and has an effect on BGSC differentiation
To ascertain that Pax3 is a negative regulator of GFAP transcription, we suppressed Pax3 expression with an siRNA that specifically targets Pax3 mRNA, while creating a Pax3 enhanced-expression model via transfection with an overexpression-Pax3 plasmid. Then, we performed RT-PCR and western blotting to determine the expression of GFAP at the mRNA and protein expression levels, respectively, with the Pax3 knockdown and overexpression BGSC models. We found that the expression of GFAP mRNA and protein was significantly greater after Pax3 knockdown compared to that noted in the untransfected cells (P<0.05). In addition, GFAP mRNA and protein were both decreased in the Pax3-overexpression model (P<0.05). The results implicate that Pax3 negatively regulates the expression of GFAP at both the mRNA and protein levels (Fig. 4). To determine whether overexpression and suppression of Pax3 modulated the differentiation of BGSCs, we transfected siRNA and an overexpression-Pax3 plasmid into the BGSCs. We performed immunofluorescence with anti-GFAP and showed that the proportion of GFAP-positive cells was 20, 24 and 67% in the negative controls, untransfected cells and BGSCs transfected with siPax3, respectively. We also observed that, in association with Pax3 silencing via siRNA, the expression of GFAP significantly increased compared to the untransfected cells (P<0.05; Fig. 5A). Furthermore, western blotting also showed that the expression of GFAP protein in the BGSCs was significantly increased after the knockdown of Pax3 compared to the untransfected cells (P<0.05; Fig. 5B). These results demonstrated that Pax3 negatively regulates the expression of GFAP and affects the differentiation in BGSCs.
Discussion
Brain glioma stem cells (BGSCs) were initially isolated from leukemic cells (19). Following Reya et al recognition of the similarities in the biological hallmarks of stem and tumor cells, it was proposed that cancers may evolve from a subset of precursor stem cells (20). Since then, stem cells have been isolated from the tumor microenvironment of numerous types of cancers, including those of the nasopharynx, breast and prostate cancer (21). Although Ignatova et al previously reported on the isolation of BGSCs from cortical glial tumors (22), it is apparent that we currently know very little in regards to the contribution of BGSCs to tumorigenesis. Accordingly, the present study endeavored to investigate the putative roles of BGSCs, with particular prominence on their contribution to the hallmarks of cancers.
CD133+ cells exist in various tissues, including umbilical cord blood, fetal brain, fetal liver and placental trophoblasts. Moreover, immunohistochemical staining has shown that CD133 is distributed throughout stem cells; on the membrane and within the cytoplasm. Recent studies have shown that CD133 is expressed in neural stem cells (NSCs) (23,24). Furthermore, nestin, a protein marker for NSCs, is also expressed in follicle stem cells. In the present study, by immunohistochemical staining, we identified CD133 and nestin as putative markers of BGSCs.
Prior research has implicated that Pax3 binds to the promoter region of GFAP, thereby negatively regulating GFAP expression and subsequently arresting the differentiation of astrocytes from NSCs (13). Furthermore, the overexpression of Pax3 has been observed within glioma tissues, in which it was reported to regulate GFAP expression in glioma cells (15). However, no studies have focused on the transcriptional relationship between Pax3 and GFAP in BGSCs. Herein, we found that Pax3 was expressed at a higher level in BGSCs than in U87MG malignant glioma cell and 1800 normal astrocyte lines. Then, we identified a binding element within the promoter region of GFAP to which Pax3 could associate, and subsequently demonstrated that Pax3 inhibits the transcription of GFAP in BGSCs.
To describe the influence of Pax3 on the behavior of BGSCs, Pax3 was silenced via the transfection of small interfering RNA (siRNA) into BGSCs. The subsequent cell proliferation, invasive and apoptosis assays showed that this siRNA-induced downregulation of Pax3 inhibited proliferation, induced apoptosis and decreased the invasiveness of transfected BGSCs. In contrast, upregulation of Pax3 via transfection of BGSCs with an overexpression vector induced increased cell proliferation and invasiveness, while suppressing apoptosis. Together, these results suggests that Pax3 plays a vital role in the growth and evolution of BGSCs.
To further determine the effects of Pax3 on BGSC differentiation and GFAP expression, siPax3-transfected BGSCs were cultivated in culture medium containing serum, to which the ability of BGSCs to differentiate was decreased. To the contrary, differentiation was increased in the overpression Pax3 plasmid-transfected BGSCs. Our results indicate that Pax3 acts as a transcriptional repressor during serum-induced differentiation of BGSCs. Thereby, it is reasonable to speculate that Pax3 suppresses the expression of GFAP during oncogenesis.
In conclusion, we firstly demonstrated that Pax3 binds to the promoter region of GFAP, and consequently negatively regulates GFAP expression in BGSCs. Pax3 can be considered a regulator of BGSC differentiation and may determine the degree of the malignancy of gliomas. Pax3 also plays a crucial role in the regulation of the growth and invasion of BGSCs. The results of the present study imply that Pax3 is a putative target for novel therapies endeavoring to treat gliomas.
Acknowledgments
Brain glioma stem cells were kindly gifted by Soochow University, China. The present study was supported by the Natural Science Foundation of Jiangsu Province (BK20130386), the National Natural Science Foundation of China (81402447), the Chinese Projects for Postdoctoral Science Funds (no. 2015M571792), the Jiangsu Planned Projects for Postdoctoral Research Funds (no. 1402200C), the Six Major Human Resources Project of Jiangsu Province (2014-WSW-028), and the Technology Project of Nantong (HS2014053).
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