Thoracic Ganglioneuroma: A Rare Neural Tumor (Case Report and Literature Review)

Ganglioneuroma is an extremely rare tumor that is derived from neural crest. Many ganglioneuroma cases are detected incidentally unless they are large enough to cause compressive symptoms. We report an 18-year-old patient with posterior mediastinal ganglioneuroma which was abutting the descending aorta. The patient underwent successful resection by thoracoscopic approach and was followed up for one year with no complications. In summary, a detailed review with experts in both radiology and pathology is mandated to diagnose these tumors. Informed consent was obtained from the patient.

Similarity on neural stem cells and brain tumor stem cells in transgenic brain tumor mouse models

Although it is believed that glioma is derived from brain tumor stem cells, the source and molecular signal pathways of these cells are still unclear. In this study, we used stable doxycycline-inducible transgenic mouse brain tumor models （c-myc/SV40Tag＋/Tet-on＋） to explore the malignant trans- formation potential of neural stem cells by observing the differences of neural stem cells and brain tumor stem cells in the tumor models. Results showed that chromosome instability occurred in brain tumor stem cells. The numbers of cytolysosomes and autophagosomes in brain tumor stem cells and induced neural stem cells were lower and the proliferative activity was obviously stronger than that in normal neural stem cells. Normal neural stem cells could differentiate into glial fibrillary acidic protein-positive and microtubule associated protein-2-positive cells, which were also negative for nestin. However, glial fibrillary acidic protein/nestin, microtubule associated protein-2/nestin, and glial fibrillary acidic protein/microtubule associated protein-2 double-positive cells were found in induced neural stem cells and brain tumor stem cells. Results indicate that induced neural stem cells are similar to brain tumor stem cells, and are possibly the source of brain tumor stem cells.

Upregulation of stromal cell-derived factor-1 alpha/CXCR4 axis-induced migration of human neural progenitors by tumor necrosis factor-alpha and interleukin-8

BACKGROUND： Studies of several animal models of central nervous system diseases have shown that neural progenitor cells （NPCs） can migrate to injured tissues. Stromal cell-derived factor 1 alpha （SDF-la）, and its primary physiological receptor CXCR4, have been shown to contribute to this process. OBJECTIVE： To investigate migration efficacy of human NPCs toward a SDF-1α gradient, and the regulatory roles of tumor necrosis factor-α （TNF-α） and interleukin-8 （IL-8） in SDF-1α/CXCR4 axis-induced migration of NPCs. DESIGN, TIME AND SETTING： An in vitro, randomized, controlled, cellular and molecular biology study was performed at the Laboratory of Department of Cell Biology, Medical College of Soochow University between October 2005 and November 2007. MATERIALS： SDF-1α and mouse anti-human CXCR4 fusion antibody were purchased from R＆D Systems, USA. TNF-αwas purchased from Biomyx Technology, USA and IL-8 was kindly provided by the Biotechnology Research Institute of Soochow University. METHODS： NPCs isolated from forebrain tissue of 9 to 10-week-old human fetuses were cultured in vitro. The cells were incubated with 0, 20, and 40 ng/mL TNF-α, or 0, 20, and 40 ng/mL IL-8, for 48 hours prior to migration assay. For antibody-blocking experiments, cells were further pretreated with 0, 20, and 40 μg/mL mouse anti-human CXCR4 fusion antibody for 2 hours. Subsequently, the transwell assay and CXCR4 blockade experiments were performed to evaluate migration of human NPCs toward a SDF-1α gradient. Serum-free culture medium without SDF-1α served as the negative control. MAIN OUTCOME MEASURES： The transwell assay was performed to evaluate migration of human NPCs toward a SDF-1α gradient, which was blocked by fusion antibody against CXCR4. In addition, CXCR4 expression in human NPCs stimulated by TNF-α and IL-8 was measured by flow cytometry. RESULTS： Results from the transwell assay demonstrated that SDF-1α was a strong chemoattractant for human NPCs （P 〈 0.01）, and 20 ng/mL produced the highest levels of migration. Anti-human CXCR4 fusion antibody significantly blocked the chemotactic effect （P 〈 0.05）. Flow cytometry results showed that treatment with TNF-α and IL-8 resulted in increased CXCR4 expression and greater chemotaxis efficiency of NPCs towards SDF-1α（P 〈 0.01）. CONCLUSION： These results demonstrated that SDF-la significantly attracted NPCs in vitro, and neutralizing anti-CXCR4 antibody could block part of this chemotactic function. TNF-α and IL-8 increased chemotaxis efficiency of NPCs towards the SDF-1αgradient by upregulating CXCR4 expression in NPCs.

Establishment and expression of recombinant human glial cell linederived neurotrophic factor and TNF α receptor in human neural stem cells

Objective:To investigate the interference and expression of human glial cell line-derived neurotrophic factor(hCDNF) and soluble TNF alpha(sTMFRⅠ) receptor genes in neural stem cells and to evaluate the roles of these proteins in the genetic treatment of spinal cord injury.Methods:Full-length of GDNF cDNA(538 bp) and sTMFRⅠcDNA(504 bp) were inserted into the early 1 region of adenovirus genomic DNA respectively and were immediated by the human cytomegalovirus(gene promoter/enhancer). These adenoviruses were propagated in HEK293 cells via homologous recombination for 7-10 days in vivo,then they were used to infect human neural stem ceils.The infection and expression of gene were tested under immunofluorescence.ELISA and Westem-blot after 48 hours.Results:Almost all the cultured cells showed the nestin immunofluorescence positive staining,which was the characteristics of neural stem cell.A great quantity of EGFP and KFP were observed in neural stem cells,which indicated the expression of GDNF and sTMFRⅠ.After transfection of GDNF and sTMFRⅠgenes,many neural stem cells show GFAP and tubulin immunofluorescence positive staining,which meant that most neural stem cells differentiated into neuron at that condition.Conclusions:The infective efficiency of adenovirus is greatly acceptable to neural stem cell,thus adenovirus provide a useful vector for exogenous GDNF and sTMFRⅠgenes expressing in neural stem cells,which is useful for differentiation of neural stem cell.

Mechanisms of hepatocellular carcinoma progression

Hepatocellular carcinoma(HCC) is the most common primary malignancy of the liver. It is the second leading cause of cancer-related deaths worldwide, with a very poor prognosis. In the United States, there has been only minimal improvement in the prognosis for HCC patients over the past 15 years. Details of the molecular mechanisms and other mechanisms of HCC progression remain unclear. Consequently, there is an urgent need for better understanding of these mechanisms. HCC is often diagnosed at advanced stages, and most patients will therefore need systemic therapy, with sorafenib being the most common at the present time. However, sorafenib therapy only minimally enhances patient survival. This review provides a summary of some of the known mechanisms that either cause HCC or contribute to its progression. Included in this review are the roles of viral hepatitis, non-viral hepatitis, chronic alcohol intake, genetic predisposition and congenital abnormalities, toxic exposures, and autoimmune diseases of the liver. Well-established molecular mechanisms of HCC progression such as epithelial-mesenchymal transition, tumor-stromal interactions and the tumor microenvironment, cancer stem cells, and senescence bypass are also discussed. Additionally, we discuss the roles of circulating tumor cells,immunomodulation, and neural regulation as potential new mechanisms of HCC progression. A better understanding of these mechanisms could have implications for the development of novel and more effective therapeutic and prognostic strategies, which are critically needed.

CXCR4-Expressing Glial Precursor Cells Demonstrate Enhanced Migratory Tropism for Glioma

Malignant glioma remains one of the most intractable of human cancers principally due to the highly infiltrative nature of these neoplasms. The use of neural precursor cells (NPC) has received considerable attention based on their ability to selectively migrate towards disseminated areas of tumor in vivo and their described ability to deliver tumor-directed therapies specifically to infiltrating tumor cells. Fundamental to optimizing the use of these cells for potential clinical translation is the development of an understanding regarding the biologic cues that govern their ability to migrate towards infiltrative glioma foci. To this end, in this paper we detail that NPC selected for double-expression of the glial-precursor marker A2B5 and the cell-surface chemokine receptor, CXCR4, demonstrate enhanced in vitro gliomadirected tropism. These findings demonstrate the relevance of these markers for the phenotypic segregation of an optimally tumor-tropic NPC sub-population as a means of enhancing NPC-based therapeutic strategies for the treatment of glioma.

基于病理组织切片的肺腺癌肿瘤突变负荷预测模型

肺癌是目前死亡率最高的恶性癌症之一,其中非小细胞肺癌(NSCLC)致死率极高。最近医学研究发现,肿瘤突变负荷(TMB)对于癌症的免疫治疗和化疗的疗效具有较好的预测作用,但传统使用基因测序计算TMB的方法存在检测成本高、周期长、样本依赖度高等缺点。针对上述问题,本研究提出一种混合卷积神经网络和自注意力机制的深度学习模型(FCA-Former)用于预测TMB。该模型以CoAtNet为骨干网络,通过在网络中结合坐标注意力以及融合深度可分离卷积的方式,提高模型的运算速度以及对病理组织切片图像的全局特征提取能力。实验数据采用TCGA数据库中肺腺癌数字病理切片图像数据集,其中高TMB水平的样本271张,低TMB水平的样本66张。实验结果表明,所提方法达到的最高平均曲线下面积(AUC)为98.1%,比现有最好方法RcaNetr提高9.8%。此项研究结果对于NSCLC的预后治疗效果具有较强的指导意义。

LncRNA NEAT1调节微小RNA-144-3p/NOVA1轴对高糖诱导的人视网膜微血管内皮细胞损伤的影响

目的探究长链非编码RNA(long non-coding RNA,LncRNA)核富含丰富的转录本1(nuclear-enriched abundant transcript 1,NEAT1)通过微小RNA(micro RNA,miR)-144-3p/神经肿瘤腹侧抗原1(neural tumor ventral antigen 1,NOVA1)对高糖诱导的人视网膜微血管内皮细胞(human retinal microvascular endothelial cells,hRMECs)损伤的影响。方法将h RMECs分为高糖组(不转染)、对照组(不转染)、高糖+si-NEAT1-阴性对照(negative control,NC)组(转染siRNA-NC)、高糖+si-NEAT1组(转染NEAT1 siRNA)、高糖+si-NEAT1+抑制剂-NC组(共转染NEAT1 siRNA+抑制剂-NC)、高糖+si-NEAT1+miR-144-3p抑制剂组(共转染NEAT1 siRNA+miR-144-3p抑制剂)、高糖+si-NOVA1-NC组(转染NOVA1 siRNA-NC)、高糖+si-NOVA1组(转染NOVA1 siRNA)。实时荧光定量聚合酶链反应技术(real-time fluorescent quantitative polymerase chain reaction,qRT-PCR)检测hRMECs中NEAT1、miR-144-3p表达量;CCK-8、Transwell和血管形成实验分别分析hRMECs增殖、迁移和血管形成能力;双荧光素酶报告实验分析NEAT1与miR-144-3p、miR-144-3p与NOVA1的结合情况;Western blot检测NOVA1、VEGF蛋白表达。结果与对照组比较,高糖组hRMECs中NEAT1表达(2.67±0.13 vs.1.02±0.08)、相对活力、迁移数量[(271.50±20.35)个vs.(144.30±16.41)个]、成管节点数[(426.50±22.75)个vs.(181.70±12.43)个]、管长度[(12725.46±136.57)μm vs.(8009.32±107.32)μm]均较高,miR-144-3p表达(0.46±0.06 vs.1.00±0.05)较低,差异有统计学意义(P<0.05)。敲低NEAT1可明显下调h RMECs中NEAT1的表达,上调miR-144-3p的表达,同时降低NOVA1(0.80±0.09 vs.1.35±0.07)、血管内皮生长因子(vascular endothelial growth factor,VEGF)蛋白表达及hRMECs的相对活力、迁移数量[(231.60±14.25)个vs.(271.50±20.35)个]、成管节点数[(234.30±13.18)个vs.(426.50±22.75)个]和管长度[(9208.74±130.85)μm vs.(12725.46±136.57)μm],差异有统计学意义(P<0.05),上述作用可被miR-144-3p抑制剂减弱。NEAT1可结合并下调miR-144-3p表达,且NOVA1为miR-144-3p的靶基因。敲低NOVA1可明显降低hRMECs相对活力、迁移数量、成管节点数、管长度,差异有统计学意义(P<0.05)。结论敲低NEAT1可上调miR-144-3p表达,下调NOVA1蛋白表达,进而抑制hRMECs增殖、迁移和血管形成能力。

血清NCAM sTNFR1水平与超时间窗后循环脑卒中患者接受替罗非班治疗后神经预后的关系分析

目的探讨血清神经细胞黏附分子(NCAM)、可溶性肿瘤坏死因子受体1(sTNF-R1)水平与超时间窗后循环脑卒中(APCIS)患者接受替罗非班治疗后神经预后的关系。方法选择2019-03—2022-01唐山中心医院收治的100例超时间窗APCIS患者(APCIS组)和63例健康体检志愿者(对照组),根据NIHSS评分将APCIS患者分为轻度损伤组(<6分,27例)、中度损伤组(6~13分,39例)、重度损伤组(≥14分,34例)。所有患者入组后均接受替罗非班经微导管动脉给药[0.4μg/(kg·min)]和静脉持续泵注[0.1μg/(kg·min)]治疗48 h,配合降脂以及双抗血小板治疗。检测血清NCAM、sTNF-R1水平,出院后定期随访90 d,统计随访期间不良神经预后发生情况。多因素Logistic回归分析APCIS患者接受替罗非班治疗后神经预后不良的危险因素,受试者工作特征曲线(ROC)分析NCAM、sTNF-R1预测APCIS患者接受替罗非班治疗后神经预后不良的价值。结果APCIS组血清NCAM、sTNF-R1水平高于对照组(P<0.05),重度损伤组血清NCAM、sTNF-R1水平高于中度损伤组和轻度损伤组(P<0.05),预后不良组血清NCAM、sTNF-R1水平高于预后良好组(P<0.05)。房颤、高NIHSS评分、高NCAM、高sTNF-R1是APCIS患者接受替罗非班治疗后神经预后不良的危险因素(P<0.05)。NCAM、sTNF-R1预测APCIS患者接受替罗非班治疗后神经预后不良的曲线下面积为0.698、0.770,联合预测曲线下面积为0.937,高于单独指标预测(P<0.05)。结论APCIS患者血清NCAM、sTNFR-1水平增高,且与APCIS神经缺损程度以及替罗非班治疗后神经预后不良有关。

毛囊表皮神经嵴干细胞调节面神经损伤后局部炎症因子的表达水平

背景:既往研究报道了毛囊表皮神经嵴干细胞在周围神经修复中的巨大潜力,但其炎症调节作用在面神经修复研究中鲜有报道。目的:探究毛囊表皮神经嵴干细胞能否调节面神经损伤后早期局部肿瘤坏死因子α和白细胞介素4表达水平,以促进面神经功能和形态恢复。方法:提取4 d龄SD大鼠毛囊表皮神经嵴干细胞进行培养、鉴定。取54只成年雄性SD大鼠制备面神经干缺损自体静脉导管桥接模型,随机等分为生理盐水组、DMEM组和毛囊表皮神经嵴干细胞组。通过免疫蛋白印迹、免疫组化、免疫荧光观察术后4-14 d肿瘤坏死因子α和白细胞介素4表达水平。对术后12周大鼠进行面神经功能评分,并行苏木精-伊红染色观察面神经形态。结果与结论:(1)毛囊表皮神经嵴干细胞中Nestin和p75NTR双阳性表达,细胞纯度>90%;(2)与其他两组相比,毛囊表皮神经嵴干细胞组的肿瘤坏死因子α表达在术后7 d减弱(P<0.05),而白细胞介素4表达在术后3,7,14 d均增强(P<0.05);(3)与其他两组相比,毛囊表皮神经嵴干细胞组的面神经功能改善(P<0.05);(4)面神经移植段均可见新生血管和再生轴突,与其他两组相比,毛囊表皮神经嵴干细胞组移植段和移植远段的神经纤维排列更有序、包绕的髓鞘更厚;(5)结果表明:毛囊表皮神经嵴干细胞对面神经损伤后修复早期局部肿瘤坏死因子α和白细胞介素4表达具有调节作用,可抑制局部炎症反应,并促进面神经功能和形态恢复。

稀土化合物氯化镧影响神经干细胞增殖的探讨

目的初步探讨稀土化合物氯化镧(Lanthanum chloride,LaCl3)对体外培养的NSCs增殖状况的影响。方法采用成球悬浮法分离培养小鼠神经干细胞(mNSCs);将生长状态良好的第3代mNSCs分为空白对照组、肿瘤坏死因子-α(TNF-α)组、LaCl3组,分别采用常规NSCs培养液、含10ng/ml TNF-α的NSCs培养液、含2.5μmol/L LaCl3的NSCs培养液培养NSCs1～3天。采用神经球计数、神经球体积测量方法以及采用免疫荧光细胞化学方法检测与细胞增殖相关的指标(CyclinD1)来观察NSCs的增殖状况。结果神经球计数和神经球体积测量结果显示,TNF-α组和LaCl3组神经球数量分别为[(74.56±2.6)个/瓶]和[(62.32±2.8)个/瓶],较空白对照组[(42.28±3.5)个/瓶]明显增多,P<0.05;神经球体积分别为[(0.82±0.16)×106(μm3)]和[(0.66±0.12)×106(μm3)],较对照组[(0.26±0.08)×106(μm3)]明显增大,P<0.05。免疫细胞荧光检测细胞增殖结果显示,TNF-α组和LaCl3组中,CyclinD1阳性细胞率分别为(68.6±4.2)%和(51.2±2.8)%,明显高于空白对照组的(35.6±2.6)%,P<0.01。结论一定浓度的LaCl3具有促进NSCs增殖的作用。

Hedgehog-Gli信号传导通路在脑肿瘤中的研究进展

脑肿瘤,特别是恶性脑肿瘤的治疗目前仍是临床医生面临的一个难题,重要的原因之一是由于对脑肿瘤的发生发展机制尚不明了。最新研究表明:神经干细胞、脑肿瘤干细胞都可能参与这一过程,针对干细胞水平的研究将给脑肿瘤的治疗带来新希望。Hedgehog-Gli信号通路正是一条影响干细胞生物学行为的重要通路。本文就该通路在神经系统发育、神经干细胞分化和脑肿瘤发生的研究作一综述。

CD133免疫磁珠分选脑肿瘤干细胞及其生物学特性

目的:从人脑肿瘤组织中分离、培养、纯化和鉴定脑肿瘤干细胞(BTSCs),探讨CD133免疫磁珠分选方法获取BTSCs的可行性及BTSCs的生物学特性。方法:留取人脑胶质母细胞瘤新鲜标本,分离获得脑肿瘤细胞。应用CD133免疫磁珠分选方法纯化BTSCs;流式细胞仪检测分选阳性率;神经球计数法分析CD133+/-亚群细胞神经球形成情况;免疫荧光方法检测CD133+/-亚群细胞表面神经干细胞(NSCs)标记物CD133、神经巢蛋白(nestin)表达情况;检测CD133+/-亚群细胞经诱导分化后细胞表面分化标记物β-TubulinⅢ、GFAP表达情况。结果:CD133+亚群细胞具有干细胞特性,可形成明显的神经球,具有自我更新和明显的增殖能力,并且NSCs标记物CD133、nestin表达阳性,经诱导分化后分化标记物β-TubulinⅢ、GFAP表达阳性;CD133-亚群细胞无上述特性。结论:CD133免疫磁珠分选方法获得的CD133+亚群细胞即为BTSCs,该方法可以得到高纯度的BTSCs,可以用于BTSCs的实验研究。

巢蛋白与神经干细胞

巢蛋白(Nestin)表达起始于胚胎早期神经前体细胞,在胚胎脑中呈时空序列性表达,目前主要作为神经干细胞的标记蛋白,应用于神经干细胞的分离、鉴定和培养。Nestin在中枢神经损伤后能重新表达,可作为中枢神经系统损伤的最早、快速应答的敏感指标。其在多系统肿瘤中高表达,并与肿瘤病理级别及预后相关。

胶质瘤干细胞与神经干细胞基因表达差异的微阵列基因芯片分析

目的利用基因芯片技术筛选人脑胶质瘤干细胞(GSCs)和正常神经干细胞(NSCs)中差异表达的基因。方法利用人类HOA5.1 OneArray表达谱芯片(包括29 186个基因),与GSCs和NSCs的总RNA生成的探针进行杂交,通过寡核苷酸芯片ScanArray 4000筛选两者之间的差异基因,并选择其中的部分差异表达基因(DCX、PTGS2、SCGN、GAD2、OTX2、PEG10、NRXN3)进一步行qRT-PCR验证。结果与正常NSCs相比,GSCs中1372个基因表达下调,1501个基因表达上调,功能富集分析显示,这些差异基因主要参与了神经轴突导向、细胞周期、细胞黏附、免疫炎症反应及癌症相关的信号路径。qRT-PCR检测结果与芯片检测结果相符。结论多类基因在胶质瘤的发生发展中发挥着重要作用,该结果可为胶质瘤的靶向治疗提供新的线索。

成人骨髓源性神经干细胞中抑癌基因p53、Rb1与p16突变的检测

目的对成人骨髓源性神经干细胞（Md-NSCs）中重要抑癌基因p53、Rb1及p16进行突变检测,旨在从抑癌基因方面研究Md-NSCs的致瘤性问题。方法从正常成人志愿者获取成人骨髓基质细胞（hMSCs）,于体外诱导培养获得Md-NSCs,应用PCR-DNA测序技术,PCR扩增Md-NSCs中p53基因第5-9外显子、Rb1基因第19-21外显子以及p16基因第1-2外显子,并对扩增片断进行DNA测序。结果Md-NSCs可由hMSCs于体外诱导培养简捷获取,Md-NSCs中p53基因第5-9外显子、Rb1基因第19-21外显子以及p16基因第1-2外显子的序列均与野生型一致,无发现突变现象。结论hMSCs体外诱导培养分化形成的Md-NSCs中未发现重要抑癌基因的常见突变现象,保持了遗传学的稳定性,为其体内移植的潜在致瘤性评价提供了参考依据。

神经干细胞与脑肿瘤发生

随着神经干细胞、脑肿瘤干细胞研究的深入,脑肿瘤起源于神经干细胞得到越来越多证据的支持,而传统的脑肿瘤起源及发生模式受到了前所未有的挑战。脑肿瘤神经干细胞起源学说一经证实,必将对脑肿瘤的基础研究和临床治疗指明新的方向,并带来突破性的进展。

脑星形细胞瘤中神经细胞黏附分子与PCNA的表达及其关系

目的 :研究人脑星形细胞瘤中神经细胞黏附分子 (neuralcelladhesionmolecule ,NCAM)的表达情况及其与肿瘤增殖活性 (PCNA)的相关性。方法 :收集人脑星形细胞瘤标本 48例 ,行SP法染色。结果 :正常脑组织NCAM全部表达 ,星形细胞瘤中I～II级、III级、IV级组阳性表达率分别为 95 % (1 9/ 2 0 ) ,3 8 9% (7/ 1 8)和 2 0 % (2 / 1 0 ) ,阳性细胞表达程度随肿瘤恶性程度的增高反而降低。其表达程度与PCNA免疫反应分数 (IRS)呈负相关 (r =- 0 .6 5 7,P <0 .0 5 )。结论 :随人脑星形细胞瘤恶性程度的增高 ,NCAM表达下调 ,提示NCAM表达减少参与肿瘤的生物恶性发展。

神经肿瘤干细胞在恶性胶质瘤放射治疗中的研究进展

脑胶质瘤是最常见的神经系统原发肿瘤。放射治疗是目前脑胶质瘤综合治疗最重要的治疗手段之一。然而经过放射治疗以后,部分肿瘤又会复发。随着肿瘤干细胞学说的确立,神经肿瘤干细胞的成功筛选和分离,研究者开始对其生物学特性进行了一系列基础研究,从肿瘤干细胞角度解释其放射生物学行为。放射肿瘤学研究者探求从治疗上特异于杀伤神经肿瘤干细胞,靶向作用于其相关信号转导通路,以期能为临床诊疗提供新的思路,最终使恶性胶质瘤临床放射治疗受益。

Axin基因在脑肿瘤干细胞和神经干细胞中的表达及其多态性研究

目的观察Axin基因在脑肿瘤干细胞和神经干细胞中的表达及其多态性,为临床治疗脑肿瘤疾病提供实验依据。方法取大鼠神经干细胞及胶质瘤肿瘤干细胞,采用RT-PCR、基因测序等方法研究Axin基因在脑肿瘤干细胞和神经干细胞中的表达,对反应产物进行测序,观察两组之间的序列差异,并与Genebank Axin基因序列进行比较。结果相差显微镜下观察,呈悬浮状态的脑肿瘤干细胞聚集在一起的小球,随着培养时间的延长,小球数量增多,球体不断增大但并不均一,长出的新球体大小均一,数量多。分离原代的神经干细胞形成细胞球。脑肿瘤干细胞中Axin序列的表达与神经干细胞及Genebank中Axin比较差异性很大,其相似性为75.6(。结论Axin基因在神经干细胞中正常表达,而在脑肿瘤干细胞中表达过低,说明Axin在脑肿瘤细胞增殖中起着重要的抑制作用。