Exploring Long Noncoding RNAs in Glioblastoma: Regulatory Mechanisms and Clinical Potentials

Gliomas are primary brain tumors presumably derived from glial cells. The WHO grade IV glioblastoma (GBM), characterized by rapid cell proliferation, easily recrudescent, high morbidity, and mortality, is the most common, devastating, and lethal gliomas. Molecular mechanisms underlying the pathogenesis and progression of GBMs with potential diagnostic and therapeutic value have been explored industriously. With the advent of high-throughput technologies, numerous long noncoding RNAs (lncRNAs) aberrantly expressed in GBMs were discovered recently, some of them probably involved in GBM initiation, malignant progression, relapse and resistant to therapy, or showing diagnostic and prognostic value. In this review, we summarized the profile of lncRNAs that has been extensively investigated in glioma research, with a focus on their regulatory mechanisms. Then, their diagnostic, prognostic, and therapeutic implications were also discussed.


Introduction
The WHO grade IV glioblastoma (GBM), characterized by high recurrence rate, high morbidity, and mortality, is the most common, aggressive, and deadly primary intracranial tumor in adults, reflecting the urgent need to develop new diagnostic and therapeutic targets for this devastating disease [1][2][3]. The standard therapy for GBM is the combination of maximal surgical tumor resection, radiotherapy, and chemotherapy [1,4]. However, the average life expectancy for GBM patients is only approximately 15 months after initial diagnosis even though optimal treatment has been received [5,6]. GBM malignancy and poor prognosis are closely correlated with the deregulation of signaling pathways controlling tumor cell proliferation, resistance to apoptosis, invasion, angiogenesis, and immune evasion [6,7]. Thus, investigations revealing essential molecular mechanisms governing these features of glioblastoma with potential diagnostic and therapeutic value have drawn remarkable attention [8]. With the advent of high-throughput technologies, a wide variety of noncoding RNAs, including microRNAs and long noncoding RNAs (lncRNAs), has been identified in glioma tissues and cell lines, some of which show strong functional indications [9]. Interestingly, the so-called glioma stem cells (GSCs), which are believed to be responsible for GBM initiation, therapy-resistant, and relapse, carry diverse molecular and genetic changes, including aberrant lncRNA expression [10,11]. Additionally, the competitive regulatory network formed among lncRNAs, protein-coding transcripts, and microRNAs seems to play a crucial regulatory role in the proliferation, metastasis, and resistance to apoptosis of GSCs [12][13][14]. Although researches of lncRNAs in GBMs are still in infancy, exploring their roles and mechanisms would not only deepen our understandings on molecular features of GBMs but also open new windows for unveiling novel diagnostic and therapeutic targets [15]. Here, we summarize recent progress regarding GBM-associated lncRNAs that have been under intensive investigations, with emphases on their regulatory mechanisms and clinical relevance. documented in the epigenetic regulation of X chromosome inactivation during embryogenesis [16,17]. Occasionally, functional short peptides can be derived from lncRNAs [18,19]. Until now, the NONCODE database has annotated 87,774 and 96,308 lncRNA genes in the mouse and human genome, respectively, which are far more than proteincoding genes (PCGs) [20]. LncRNA genes are largely categorized according to their locations and transcription orientations relative to the closest protein-coding genes. Thus, they can be antisense (partially or fully overlapped with PCGs), sense, divergent, convergent, intronic, and intergenic (no PCGs within a 5-kilobase range) [21]. Compared to protein-coding mRNAs, lncRNAs transcribed from intergenic regions (lincRNAs) are less spliced and largely nonpolyadenylated and are mostly attached to chromatin [22]. LncRNAs are usually expressed at lower levels than protein-coding mRNAs and display more cell typeand tissue-specific expression patterns. Notably, about 40% of lncRNAs are mainly expressed in the brain, reflecting the cellular and functional complexity of the brain [23]. Furthermore, lncRNA expression is spatiotemporally regulated during neural development [24][25][26][27] and upon neural activity [28,29]. Since many lncRNAs are capable of forming a complex with DNA, RNA, and proteins dynamically, they regulate gene expression at multiple levels including chromatin remodeling, histone and DNA modification, and the process of transcription, as well as RNA splicing, transport, and stability [6,[30][31][32][33]. Particularly, lncRNAs could play cis-regulatory roles to positively or negatively control the transcription of neighboring PCGs [34]. Although functions of most lincR-NAs have yet to be unveiled, some have been found to facilitate the chromatin structure and histone modifications, to act as a coactivator or corepressor in the nucleus [35,36] or to modulate signal transduction in the cytosol [37]. In addition, some lncRNAs bear complementary sites (also known as miRNA response elements, MRE) for microRNAs (miRNAs). miRNAs have been widely recognized to be involved in almost every facet in the development and malignant progression of gliomas, including the maintenance of the stemness of GSCs, invasiveness, angiogenesis, epigenetic regulation, and signaling pathways [38][39][40][41][42]. The so-called competitive endogenous RNAs (ceRNAs) function as molecular "sponges" for miRNAs via their MREs, thus derepressing the target genes of the respective miRNAs [43][44][45]. Circular RNAs or transcripts of pseudogenes might also behave as ceRNAs. Some studies further indicated that a few lncRNAs could modulate gene expression and/or cell signaling at multiple molecular levels simultaneously [46,47]. Given the broad involvement of lncRNAs in cellular events, it is not surprising to reveal that a number of lncRNAs play pivotal roles in embryogenesis, tissue homeostasis, and the development and progression of various diseases [48][49][50][51].

Aberrant lncRNA Expression in Glioblastomas
Dysregulated expression of lncRNAs is associated with human diseases such as cardiovascular diseases, neurodegenerative disorders, and malignant tumors, which are also evident in brain tumors [52,53]. Moreover, several studies showed that abnormal expression profiles of lncRNA in clinical glioma specimens are correlated with histological differentiation and malignancy grades, which may have clinical implications in the diagnosis and prognostication [54,55].
A high-throughput screen study by Han et al. identified 1308 differentially expressed lncRNAs in GBMs compared to normal brain tissue. Among them, ASLNC22381 and ASLNC2081 were predicted to be involved in the recurrence and malignant progression of GBM by upregulating the expression of IGF-1 (insulin-like growth factor 1) [56]. Similarly, a transcriptome comparison study identified differentially expressed lncRNAs and mRNAs between GBM and normal brain samples. Gene ontology (GO) and pathway analysis-predicted genes involved in GBM pathogenesis could be modulated by lncRNAs, such as the HOX clusterassociated lncRNAs [57]. In another study, Zhang et al. identified 129 differentially expressed lncRNAs in glioma tissues. Their analysis revealed that the levels of lncRNA MEG3 were significantly downregulated in GBMs, whereas those of HOTAIRM1 (HOX antisense intergenic RNA myeloid 1) and CRNDE were upregulated [58]. Importantly, the expression pattern of these lncRNAs correlates with histological classification and malignancy grades of gliomas [58]. Although mechanistic evidence remains to be explored, differentially expressed lncRNAs could be a start point for digging out novel biomarkers for diagnosis or targets for therapy [6]. Next, we will list individual lncRNAs regarding their involvements in multiple aspects of GBMs. In the past few years, researchers largely focused on a few well-documented, abundantly expressed lncRNAs that have explicit indications for their participation in development and/or in tumorigenesis, with some of which showing diagnostic and prognostic potentials (Table 1).

HOTAIR (HOX Transcript Antisense Intergenic RNA).
LncRNA HOTAIR, located at chromosome 12q13, was originally implicated in epigenetic silencing of genes at the HOXD locus and inhibits initiation of transcription by recruiting PRC2 (polycomb repressive complex 2) [59,60]. Aberrant HOTAIR expression was closely related to cancer metastasis and was defined as a negative prognostic factor for patients with malignant tumor [61,62]. HOTAIR expression in GBMs is significantly higher than that in normal brain tissues and low-grade gliomas and correlated with poor prognosis and glioma molecular subtype. Moreover, HOTAIR was an independent prognostic factor in GBM patients. A gene set enrichment analysis (GESA) revealed that HOTAIR expression primarily associated with genes involved in cell cycle progression. Consistently, HOTAIR maintains proliferation and tumorigenic potential of GBM cells [63]. HOTAIR regulates cell cycle progression of GBM cells probably through EZH2, the core component of the PRC2 (polycomb repressive complex 2) [64], and the Wnt/ β-catenin pathway [65]. Reports also suggest that HOTAIR might behave as a competing endogenous RNA (ceRNAs) to regulate the levels of prooncogenic transcripts by buffering miRNAs [66,67]. The mechanisms underlying elevated HOTAIR expression in glioma remain to be investigated,  [134][135][136] and a study in breast cancer hints at both transcription and posttranscriptional regulations [47]. In summary, these findings reveal that HOTAIR may enhance the development of GBM through multiple regulatory signals, and its clinical value awaits further study.

CRNDE (Colorectal Neoplasia Differentially Expressed).
LncRNA CRNDE is initially identified to be overrepresented in >90% of colorectal adenomas and adenocarcinomas [68,69]. Later, CRNDE was also found to be highly expressed in brain cancers including GBM and astrocytomas [55,69,70]. Applying a microarray-mining approach, Zhang et al. reported that CRNDE was upregulated by 32-fold up in glioma tissues than that in nontumor brain tissues [58]. CRNDE overexpression promotes glioma cell growth and migration in vitro and tumorigenesis in a xenograft mouse model. Mechanistic studies suggested that CRNDE expression could be regulated by the mTOR signaling and the histone acetylation status in the promoter region [71]. CRNDE is enriched in the stem-like population of GBM cells and promotes tumor cell proliferation and migration and by sponging down miR-186 to derepressing the expression of XIAP (X-linked inhibitor of apoptosis) and PAK7 [p21 protein-(Cdc42/Rac-) activated kinase 7], two prooncogenic molecules [72]. Similarly, CRNDE behaves ceRNAs for miR-384 to maintain the expression of PIWIL4 (piwi-like RNAmediated gene silencing 4), which promotes gliomagenesis probably by activating the STAT3 signaling [73]. Moreover, high CRNDE expression correlates with tumor progression and poor survival for glioma patients [55].

NEAT1 (Nuclear-Enriched Abundant Transcript 1).
LncRNA NEAT1 is crucial for the formation of paraspeckles, nuclear domains implicated in mRNA nuclear retention, and splicing [74][75][76]. NEAT1 is upregulated in human GBM tissues [6] and glioma cell lines like U251 and U87 [77]. NEAT1 expression was higher in glioma tissues than adjacent noncancerous tissues. Higher NEAT1 expression correlated with a larger tumor size, higher WHO grade, recurrence rate, and unfavorable overall survival, supporting NEAT1 as a potential prognostic predictor of glioma patients [78]. NEAT1 has been implicated in gliomagenesis by promoting cell proliferation, invasion, and migration. Zhen et al. demonstrated that NEAT1 could upregulate the expression of c-Met oncogene through buffering miR-449b-5p, a negative regulator of c-Met [79]. The latest study by Chen et al. showed NEAT1 could be upregulated by the oncogenic EGFR pathway. Elevated NEAT1 promotes GBM tumorigenesis by acting as a scaffold molecule to recruit the histone modification enzyme EZH2 to silence target-specific genes including AXIN2, ICAT, and GSK3B, thus leading to the activation of the canonical Wnt/β-catenin signaling. This study highlights the epigenetic role of lncRNAs in controlling the expression of tumorigenic components in GBM cells [80].

XIST (X-Inactive Specific Transcript).
LncRNA XIST is the major effector of X inactivation in mammals to balance gene expression between the sexes, and the XIST RNA is exclusively transcribed from the inactive X chromosome [16,17]. XIST loss in female mice leads to a highly aggressive myeloproliferative neoplasm and myelodysplastic syndrome (mixed MPN/MDS) [81]. XIST has been found to be up-or downregulated in a variety of human cancers [82]. Yao et al. found XIST expression was upregulated in glioma tissues and GSCs and knockdown of XIST suppresses GSC proliferation, migration, invasion, and tumorigenic potential by upregulating miR-152 [14]. A few other studies also indicated XIST confers glioma cell oncogenic and chemoresistant behaviors by serving as ceRNAs to suppress actions of micro-RNAs [83][84][85]. One recent study pointed out a novel role of XIST in regulating a glioma microenvironment. XIST was found to be overrepresented in glioma endothelial cells (GECs), and XIST knockdown increased permeability of the brain-tumor barrier (BTB) and inhibited glioma angiogenesis, which may have beneficial effects on GBM treatment. Mechanistically, XIST regulates the expression of the transcription factor Forkhead Box C1 (FOXC1) and Zonula occludens 2 (ZO-2), two molecules essential for maintaining the BTB integrity, by dampening miR-137 [86].
3.6. SOX2OT (SOX2 Overlapping Transcript). The genomic region that transcribes lncRNA SOX2OT contains the SOX2 gene, one of the major pluripotency regulators, in its intronic region [94]. Similar to SOX2, SOX2OT is highly expressed in embryonic stem cells and neural precursor cells but becomes downregulated upon differentiation. Elevated SOX2OT expression and the concomitant SOX2 expression were also noticed in some carcinomas with an epithelial origin, including lung, breast, and esophageal cancer [95]. The transcriptional regulation of SOX2 by SOX2OT has been highlighted in development and tumorigenic scenarios [96][97][98]. A recent study found SOX2OT is essential for proliferation, migration, invasion, and tumorigenesis of GBM stem-like cells (GSCs). The results also indicated SOX2OT might act as ceRNAs to maintain the expression of SOX3 by buffering miR-122 and miR-194-5p. Moreover, in GSCs, SOX3 functions as an oncogene and transactivates the expression of SOX2OT and TDGF-1, thus forming a positive feedback loop [99].

MEG3 (Maternally Expressed Gene 3).
LncRNA MEG3, also known as Gtl2 (gene trap locus 2) in mice, is transcribed from the imprinted maternal allele, with multiple isoforms generated by alternative splicing [100,101]. MEG3 expression is prevalent in human normal tissues, while it becomes diminished in most human tumors, and overexpression of MEG3 inhibits the growth of human cancer cells [102][103][104]. DNA methylation at the promoter or the intergenic differentially methylated region of MEG3 mediates silencing of the MEG3 gene in tumors. Ectopic MEG3 expression significantly elevates the level of tumor suppressor protein p53 in human cancer cell lines. The increased p53 level upon MEG3 overexpression is partly due to the downregulation of MDM2, an E3 ubiquitin ligase that targets p53 for degradation [105]. MEG3 is significantly downregulated in GBMs and behaves as a tumor suppressor in GBM cells in a p53dependent manner [106,107]. A recent study also suggested MEG3 might act as competing endogenous RNAs (ceRNAs) of miR-19a and miR-93 to inhibit GBM cell growth [108,109]. Li et al. provided evidence that hypermethylation at the MEG3 promoter mediated by DNMT1 controls the expression of MEG3 and subsequent p53 activity in glioma cells. Moreover, treating glioma cells with the DNA methylation inhibitor 5-AzadC inhibited the growth and promoted apoptosis of glioma cells, and its potential application in GBM animal models remains to be investigated [110].

MALAT1 (Metastasis-Associated Lung Adenocarcinoma
Transcript 1). LncRNA MALAT1, also known as NEAT2 (noncoding nuclear-enriched abundant transcript 2), was initially demonstrated to be positively associated with metastasis and shorter survival in non-small cell carcinoma (NSCLC) patients, specifically in the early stages of lung adenocarcinoma [111]. Analogous to NEAT1, MALAT1/ NEAT2 is majorly enriched in the paraspeckle, a nuclear structure essential for RNA storage and splicing [112]. But its role in alternative splicing might be species-specific [113]. In most solid tumors, MALAT1 is highly expressed and is associated with poorer clinical parameters [114]. Interestingly, studies in glioma have inconsistent results regarding roles of MALAT1. MALAT1 expression was reported to be lower in glioma tissues than that in noncancerous brain tissues, and its higher expression correlates with better patient survival, suggesting MALAT1 may serve as an independent prognostic factor and act as a tumor suppressor in glioma [115]. Accordingly, the proliferation and invasion ability of glioma cells was significantly enhanced by MALAT1 knockdown in glioma xenograft models, whereas MALAT1 overexpression had opposite effects [115]. MALAT1 might exert its tumor suppressor role by inactivation of the prosurvival ERK/MAPK signaling and/or enhance the expression of FBXW7, an antiproliferation protein [116]. However, a few other studies indicated MALAT1 has prooncogenic (tumor-promoting) roles and knockdown MALAT1 might confer beneficiary effects on glioma treatment [117][118][119]. Thus, MALAT1 could be either a positive or a negative regulator in glioma tumorigenesis depending on cellular contexts.
3.9. TUG1 (Taurine-Upregulated Gene 1). TUG1 was originally identified as a lncRNA required for the normal development of photoreceptors in the mouse retina [120]. As a chromatin-associated lncRNA, TUG1 can regulate gene expression by interacting with the polycomb repressive complex 2 (PRC2) [121]. TUG1 is extensively related to human malignancies, reported having either tumor promoting or tumor suppressing functions in different types of cancers [122][123][124]. TUG1 is expressed at significantly higher levels in GBM tissues than in normal brain tissues [125]. In GSCs, TUG1 expression is transcriptionally induced by the Notch signaling, a well-known oncogenic pathway. TUG1 maintains stemness and tumorigenic properties of GSCs by two parallel mechanisms: in the cytosol, TUG1 sponges miR-145 to maintain the expression of stemness-associated genes including SOX2 and MYC; in the nucleus, TUG1 is able to associate with the PRC2 and YY1 transcription factor to suppress differentiation [46]. This study underscores the importance of the Notch-lncRNA axis in regulating self-renewal of GSCs and proposes a rationale for targeting TUG1 as a potent therapeutic approach to treat GBMs by eradicating GSCs. TUG1 could maintain the expression of tumor suppressor PTEN by sponging off its negative regulator miR-26a, but the functional implication is not clear [125]. TUG1 was also found to be highly expressed in glioma endothelial cells (GECs). Serving as ceRNAs for miR-144 in GECs and miR-299 in GSCs, TUG1 is able to modulate blood-tumor barrier and enhance glioma-induced angiogenesis, respectively [126,127]. Therefore, depleting TUG1 in glioma cells might facilitate a microenvironment detrimental for tumor growth while beneficial for drug delivery.

CASC2 (Cancer Susceptibility Candidate 2).
LncRNA CASC2 is first identified to be transcribed from an allelic loss region at chromosome 10q26 in human endometrial cancer [128,129]. Later on, CASC2 was unveiled to be a tumor suppressor gene in endometrial, colorectal, lung, and renal cancers and gliomas, probably behaving as ceRNAs by buffering miR-21 and miR-18a, two microRNAs with oncogenic effects [9,[130][131][132][133]. The status of CASC2's low expression is positively correlated with advanced tumor grades, shorter survival time, and poorer TMZ response in glioma patients [134]. CACS2 overexpression could sensitize glioma cells to temozolomide (TMZ) cytotoxicity by upregulating PTEN protein and downregulating p-AKT protein through regulating miR-181a or by inhibiting autophagy via sponging miR-193a-5p to increase mTOR expression [135,136].

Potentials of lncRNAs in Diagnostic or Prognostic Applications
Like many other malignant tumors, the clinical diagnosis of glioma traditionally relies on symptoms, imaging findings from CT/MRI scans, and histological properties of resected tumor tissues. Recent advancement in high-throughput technology enables both clinicians and researchers to acquire genome, epigenome, transcriptome, and proteome data of tumor bulk or individual tumor cells [137][138][139]. Incorporation of these data generates molecular signatures of tumors much more comprehensively than traditional understanding. For instance, transcriptome signatures could classify GBMs into molecularly distinct subgroups including proneural and mesenchymal GBMs, which correspond to clinical and histological properties [140,141]. More importantly, the current WHO classification of tumors of the central nervous system is now defined by both histology and molecular features, the latter including IDH1/2 mutation, 1p/19q co-deletion, and histone H3 K27-mutant [142]. The inclusion of these molecular signatures is due to their explicit indications for prognosis and/or targeted therapy. Furthermore, sampling and molecular description of glioma tissues at multiloci or overtime for individual tumors could allow the understanding of the heterogeneity features of GBMs, as well as their evolving path molecularly [143][144][145]. The accumulation of this knowledge would eventually lead to design patient-tailored glioma therapeutics. As mentioned earlier, high-throughput transcriptome analyses of glioma tissues/cells identified numerous highly and/or differentially expressed lncRNAs, including MALAT1, HOXA11-AS, and CRNDE, which correlate with histological and molecular subclassification, and/or show prognostic values [15,55]. Zhang et al. carried out lncRNA profiling from 213 GBMs using data from The Cancer Genome Atlas (TCGA) database and identified six lncRNAs including KIAA0495, MIAT, GAS5, PART1, PAR5, and MGC21881, whose weighted expressions are closely associated with the overall survival of GBM patients. Further analysis demonstrated that the six-lncRNA signature was an independent risk factor for the prognosis of GBM patients [146]. Similarly, using consensus clustering of 1970 lncRNAs from the Rembrandt dataset, a study classified gliomas into three molecular subtypes called LncR1, LncR2, and LncR3. Moreover, LncR1 subtype was associated with the poorest overall survival rate, while the LncR3 subtype correlated with the best prognosis [147]. These are interesting attempts showing potential application of lncRNAs in diagnostic and prognostic purposes for gliomas ( Table 1). The drop of cost for molecular diagnosis based on high throughput techniques would greatly accelerate profiling of lncRNAs in glioma patients. These efforts will unveil practical lncRNA signatures for glioma, including their genomic, epigenetic, and expression features, which should be comparable with or even better than current molecular signatures. Nextgeneration diagnostics based on the CRISPR-Cas technique, including DETECTR (DNA endonuclease-targeted CRISPR trans reporter) [148] and SHERLOCK (specific highsensitivity enzymatic reporter unlocking) [149,150], will facilitate easier tumor detection and categorization molecularly, for example, using nucleic acids extracted from the cerebrospinal fluid (CSF). These emerging diagnostic tools will have to be robustly compared to standard diagnostics to ensure sensitivity and specificity.

Potentials of lncRNAs in Targeted Therapy against Glioma
Dismal outcomes for GBM patients are mostly due to high heterogeneity and aggressiveness of glioma cells, immuneprivileged brain environment, lack of effective treatment, and poor BBB penetration for most drugs [151]. Although aforementioned lncRNAs are suggested to regulate these aspects, most evidence regarding their roles in tumorigenesis is collected using in vitro cultured GBM cells and xenografted animal models. Thus, unbiased whole-genome screening followed by the genetic manipulation of lncRNAs in glioma animal models would identify lncRNAs with explicit oncogenic or tumor suppressing roles, which could pave the path for translational application [152,153]. Moreover, efficient delivering of small interfering RNAs (siRNAs) and antisense oligonucleotides (ASOs) that target lncRNAs in glioma mass requires advances in engineering and material science [154,155]. For instance, Katsushima et al. revealed that intravenous injection of ASOs targeting TUG1 in combination with a drug delivery system induced glioma stem cell differentiation and repressed tumor growth efficiently [46]. Alternatively, the CRISPR/Cas9-mediated editing of genome, epigenome, or RNA would be another promising approach to tackle glioma-expressed lncRNAs [156]. Notably, CRISPR/Cas9-based transcriptional activation or suppression can enhance or inhibit lncRNA expression epigenetically without modifying genomes, which could be advantageous to traditional gene-therapy approaches [157][158][159]. In addition, several epigenetic modulators that regulate oncogenic lncRNAs have recently emerged as novel therapeutic targets for GBM patients [110]. For example, Pastori et al. demonstrated that the inhibition of bromodomain protein BRD4 could alleviate the expression of oncogenic lncRNA HOTAIR in GBM patients, exerting an antiproliferation effect by inducing cell cycle arrest in GBM cells [160,161].

Conclusion
A large variety of lncRNAs has been identified to be associated with deregulated gene expression and imbalanced biological processes in GBMs. LncRNAs were involved in nearly all facets of GBM malignancy, including cell proliferation, stemness, angiogenesis, migration, invasion, tumor immune responses, relapse, and drug resistance. However, it remains to be determined if certain deregulated lncRNAs are core causal factors in tumorigenesis and progression of GBMs. Further, using state-of-the-art biochemical and molecular approaches, we are able to precisely delineate how lncRNAs control molecular machinery and cellular functions. This knowledge is imperative for devising targeted therapeutics. In addition, the complex glioma milieu composed of microvessels, immune cells, extracellular vesicles, cytokines, and neural transmitters is indispensable for GBM propagation and invasion [42,162]. Particularly, the latest progress using immune checkpoint inhibitors brings hopes for previously intractable tumors including GBMs [163,164]. Hence, future studies need to identify lncRNAs that have essential roles in regulating the fate and behavior of microenvironment components in GBMs.
In summary, the current understanding of GBM lncRNAs is only the tip of an iceberg, and continuing efforts will make possible developing novel RNA-based strategy to treat such a malignant tumor and bring new hopes for patients with GBM.