葡萄糖对神经干细胞缺氧性损伤保护作用的实验研究

目的探讨葡萄糖对神经干细胞缺氧性损伤的保护作用。方法分离培养小鼠胚胎11.5d神经干细胞。将三气培养箱的氧气浓度调至5%,以制备缺氧环境。分别在缺氧前后于无血清培养基中加入不同剂量的葡萄糖,同时设常氧常糖正常对照。通过计数克隆形成率和MTT法检测干细胞的存活和增殖情况,AnnexinⅤ-FITC/PI染色、激光扫描共聚焦显微镜观察和计算其凋亡率。结果缺氧前加入30 mmol/L葡萄糖,神经干细胞的存活率和增殖率较常糖缺氧组明显增高,但仍低于常糖常氧正常对照组。缺氧后再加入葡萄糖时,其保护作用不明显。结论缺氧前给予足够浓度的葡萄糖对神经干细胞的缺氧性损伤具有一定的保护作用。     

脑源性神经营养因子促进海马神经干细胞的存活、增殖及向神经元分化

探讨脑源性神经营养因子(brain derived neurotrophic factor, BDNF)对海马神经干细胞(neural progenitor/stem cells, NPCs)的存活、增殖及分化的影响.采用无血清培养基体外分离、纯化、扩增胎鼠海马NPCs.通过细胞形态观察、nestin免疫荧光染色及血清促分化检测NPCs的干细胞特性; 采用神经球计数及神经球直径测定观察BDNF对NPCs的促增殖作用, 筛选出在适当细胞密度下, 促进NPCs增殖的有效浓度; 采用Tunel染色及全自动生化分析仪测定细胞培养上清液乳酸脱氢酶(lactic dehydrogenase, LDH)的含量探讨BDNF对海马NPCs存活的影响; 采用抗-b-微管蛋白(tubulin) III (Tuj-1)染色检测NPCs分化成神经元的百分率, 同时测定分化神经元突起的长度.分离的海马NPCs表现为nestin 免疫染色阳性, 具有自我增殖能力、且能分化为神经元和星形胶质细胞; 当细胞密度为5×105个/ ml 时, 10～200 ng/ml BDNF能显著促进NPCs的增殖, 其中40 ng/ml BDNF促增殖作用最强, 40 ng/ml BDNF能显著增大神经球直径; 40 ng/ml BDNF 显著减少NPCs的凋亡率(Tunel /DAPI ), 抑制LDH漏出; 40 ng/ml BDNF能显著促进NPCs分化为Tuj-1免疫染色阳性神经元, 且分化后神经元的突起长度显著大于对照组.上述结果提示: BDNF促进海马NPCs的存活、增殖及向神经元方向分化.     

神经上皮干细胞的分离培养及其体外分化特性的观察

目的探讨大鼠胚胎神经管神经上皮干细胞的分离培养条件,并观察其在体外的分化特性.方法采用显微解剖、机械吹打、无血清悬浮培养方法分离培养神经上皮干细胞,采用巢蛋白(nestin)免疫细胞化学染色技术检测神经上皮干细胞,用NSE和GFAP免疫组化染色检测并计数神经细胞和神经胶质细胞.结果大鼠胚胎神经管神经上皮干细胞在无血清培养基中可形成大量呈nestin抗原阳性细胞构成的神经球,经传代有血清培养后分化为NSE阳性和GFAP阳性细胞,其中NSE阳性细胞占细胞总数的47.7%,GFAP阳性细胞占细胞总数的39.8%.结论胎鼠神经管神经上皮干细胞在无血清培养中可增殖和传代,在有血清培养中可分化为神经细胞和神经胶质细胞,两者之比为47.7∶39.8.     

钙离子与缺氧性神经干细胞凋亡的相关性研究

目的检测钙离子浓度在缺氧性神经干细胞凋亡过程中的变化,以探讨缺氧性神经干细胞凋亡的发生机制。方法从大鼠胚胎神经管获取神经干细胞,经无血清悬浮培养技术获得神经球。对所获神经球行干细胞克隆试验、Br-dU掺入标记试验、nestin、NSE和GFAP免疫荧光染色,以确认神经干细胞的生物学特性。三气培养箱予以缺氧干预,按缺氧程度分为5%O2组、10%O2组和正常对照组(20%O2),每个实验组又依缺氧干预时间的不同,分为24h、48h、72h、96h、120h5个亚组。用激光扫描共聚焦显微镜和Fluo-3荧光探针标记技术检测神经干细胞内钙离子浓度;采用An-nexinⅤ-FITC/PI检测细胞凋亡率。结果5%O2120h组和10%O2120h组中神经干细胞凋亡率显著高于正常对照组和其他缺氧干预组,并且伴随有胞内钙超载。结论细胞内钙超载可能是缺氧性神经干细胞凋亡机制中的一个重要环节。     

乳鼠海马神经干细胞的体外分离、扩增和分化研究

探讨海马神经干细胞（neuralstemcells,NSCs）在体外分离扩增和诱导分化的可行性。无菌条件下分离新生（24h）SD大鼠海马神经干细胞,采用无血清培养和胎牛血清诱导分化。免疫荧光染色技术分别检测诱导前细胞巢蛋白（Nestin）的表达,以及分化细胞的神经元特异性烯醇化酶（neuron specific enolase,NSE）、胶质纤维酸性蛋白（glialfibrillaryacidicprotein,GFAP）的表达,以鉴定细胞类型。流式细胞仪检测神经干细胞分化前后增殖能力的变化。结果显示：从乳鼠海马分离培养的细胞生长状态良好,具有克隆增殖能力,并呈Nestin表达阳性,分化后可出现NSE及GFAP表达阳性的细胞。流式细胞仪检测显示：诱导前,细胞增殖活跃,S＋G2／M期细胞为（36．27±1．99）％,而分化各阶段（3,7,10d）S＋G2／M期细胞比例与诱导前（Ctrl）相比则明显下降（尸〈0．05）,分别为（26．39±1．10）％、（26．33±1．33）％和（24．54±1．12）％。这些结果表明乳鼠海马存在神经干细胞,并具有自我更新和多向分化的潜能,可用于基础和临床的相关研究。     

胎鼠脊髓神经干细胞分离方法的比较

目的：比较机械法和胰酶消化法对胎鼠脊髓源神经干细胞增殖分化的影响。方法：分别用机械法和胰酶消化法分离胎鼠脊髓组织获得神经干细胞,应用台盼蓝检测细胞成活率,用无血清培养技术培养神经干细胞,应用MTT法检测细胞分裂增殖能力．采用免疫细胞化学法鉴定神经干细胞和分化细胞。结果：机械法获得的细胞数量多于胰酶消化法。细胞经过培养其增殖能力机械法略强于胰酶消化法,但无统计学意义。培养形成的细胞球Nestin阳性,诱导分化后可见NSE和GFAP阳性细胞。结论：运用机械法比胰酶消化法分离胎鼠脊髓组织获得神经干细胞方法简单,容易操作,经过培养细胞增殖能力较强。并可提供健康的细胞来源。     

兔胚胎神经干细胞的分离、培养和鉴别

目的：研究兔胎脑神经干细胞体外生长特性,为探讨神经干细胞的临床应用及神经系统的发育奠定基础。方法：采用含碱性成纤维细胞生长因子（bFGF）和表皮细胞生长因子（EGF）的N2无血清培养技术,取18天龄兔胚胎脑组织,分离神经干细胞,并观察分离的细胞体外培养、增殖、分化潜能,免疫组化鉴定。结果：从18天龄兔胎脑皮质和纹状体中成功分离出具有自我更新和多分化潜能的神经干细胞,在无血清培养时细胞呈半贴壁状态生长,形成神经球,可传代。细胞呈Nestin免疫反应阳性;在含血清培养基中培养时则分化,分化后的细胞表达神经元细胞、星形胶质细胞和少突胶质细胞的特异性抗原。结论：来自兔胎脑神经干细胞能在体外培养、增殖并保持传代能力。无血清N2EGF、bFGF培养基有利于兔胎脑神经干细胞的存活和增殖,含血清培养基能诱导兔胎脑神经干细胞分化。     

淫羊藿苷促进宫颈癌TC-1细胞凋亡作用的研究

目的:研究淫羊藿苷体外对致宫颈癌TC-1细胞的增殖抑制及促凋亡作用。方法:利用细胞培养,用不同浓度的淫羊藿苷在一定的时间处理致宫颈癌TC-1细胞,光学显微镜直接观察药物对细胞的作用;MTT法检测淫羊藿苷对TC-1细胞的增殖抑制作用;Dapi核染色、Annexinv-FITC/PI流式细胞学检测细胞凋亡。结果:淫羊藿苷对TC-1细胞有显著的抑制作用,且呈时间、剂量依赖,20μg/ml作用72小时后,细胞抑制率达99%;DAPI核染色和流式细胞术检测可发现典型细胞凋亡特征。结论:淫羊藿苷对TC-1细胞增殖有抑制和促凋亡作用,并呈时间浓度依赖性。     

淫羊藿苷促进宫颈癌TC-1细胞凋亡作用的研究

目的：研究淫羊藿苷体外对致宫颈癌TC-1细胞的增殖抑制及促凋亡作用。方法：利用细胞培养,用不同浓度的淫羊藿苷在一定的时间处理致宫颈癌TC-1细胞,光学显微镜直接观察药物对细胞的作用;MTT法检测淫羊藿苷对TC-1细胞的增殖抑制作用;Dapi核染色、Annexinv-FITC/PI流式细胞学检测细胞凋亡。结果：淫羊藿苷对TC-1细胞有显著的抑制作用,且呈时间、剂量依赖,20μg/ml作用72小时后,细胞抑制率达99%;DAPI核染色和流式细胞术检测可发现典型细胞凋亡特征。结论：淫羊藿苷对TC-1细胞增殖有抑制和促凋亡作用,并呈时间浓度依赖性。     

海星皂甙1对人胶质瘤U87细胞抗增殖作用的研究

目的:海星皂甙是一类从海星中分离、萃取出来的甾体苷类,被认为是海星体内毒素的主要成分.研究表明海星皂甙及其化学衍生物具有多种药理学活性,包括抗菌、抗病毒、抗肿瘤、抑制真菌活性等.本实验旨在研究海星皂甙1对人胶质瘤U87细胞的抗增殖作用和可能的机制.方法:不同浓度海星皂甙l处理人胶质瘤U87细胞后,采用MTT法检测细胞活力,TUNEL染色观察细胞凋亡情况,Westernblot检测内质网应激相关凋亡分子的活性.结果:①海星皂甙1显著抑制U87细胞的增殖,呈时间与剂量依赖性.②海星皂甙1诱导U87细胞发生凋亡.③海星皂甙1处理后U87细胞内质网相关凋亡分子活性明显增高.结论:海星皂甙1通过诱导细胞凋亡抑制人胶质瘤U87细胞的增殖,这种抗增殖作用可能是通过激活内质网应激相关凋亡分子实现的.     

缺氧培养对大鼠神经干细胞体外增殖影响及其机制的研究

目的：研究应用缺氧对体外培养的大鼠神经干细胞增殖的影响。方法：将细胞分为4小时缺氧组、12小时缺氧组、促红细胞生成素（EPO）中和抗体组、IgG组以及对照组．测定大鼠神经干细胞经缺氧培养后的各组细胞克隆形成率以及EPO的表达变化。结果：单细胞培养条件下,与对照组相比,4小时缺氧组和IgG组克隆形成率明显增高;中和抗体组无明显变化;12小时组克隆形成率降低。但无统计学意义。缺氧4小时后,EPO蛋白在预处理后即刻出现表迭,4h达高峰,8h仍有部分表达。结论：短时间缺氧可以促进神经干细胞增殖．长时间缺氧则作用相反。缺氧对NSCs增殖作用的影响可能是由EPO介导产生。     

丁酸钠对CHO-EPO工程细胞株rhEPO表达量的影响

以稳定整合有ｐＥＤＥＰＯ的ＣＨＯＥＰＯ工程细胞株为研究对象,在无血清条件下,系统观察了０５、１０、２５和５０ｍｍｏｌ／Ｌ４个浓度的丁酸钠作用于该细胞株的情况,结果表明：丁酸钠对ＣＨＯＥＰＯ工程细胞的生长有明显的抑制作用;影响ＣＨＯＥＰＯ工程细胞ＥＰＯ表达,浓度１０ｍｍｏｌ／Ｌ可提高ＥＰＯ表达量２５倍左右,并可持续较长的一段时间;延缓ＣＨＯＥＰＯ工程细胞在无血清培养时的细胞脱落;提高ＣＨＯＥＰＯ工程细胞ＥＰＯｍＲＮＡ水平     

Beneficial effect of silkworm hemolymph on a CHO cell system: Inhibition of apoptosis and increase of EPO production

To produce erythropoietin (EPO), Chinese hamster ovary (CHO) cells were first cultured in a medium containing FBS (growth medium) and then in a serum-free medium containing sodium butyrate (production medium). Sodium butyrate increases recombinant protein production, but also induces apoptosis, which reduces cell viability and productivity. In a previous study, we found that silkworm hemolymph (SH), an insect serum, inhibits the apoptosis of insect and mammalian cells. To overcome sodium butyrate-induced apoptosis, we added SH to growth medium. This pretreatment with SH inhibited the sodium butyrate-induced apoptosis of CHO cells and consequently increased their longevity and their ability to produce EPO. As a result, the volumetric productivity of EPO was increased five-fold. SH was found to inhibit cytochrome c release from mitochondria into the cytosol, and prevented the activation of caspase-3 and other subsequent caspase reactions.     

Expression of GD2 and GD3 gangliosides in human embryonic neural stem cells

NSCs (neural stem cells) are undifferentiated neural cells endowed with a high potential for proliferation and a capacity for self-renewal with retention of multipotency to differentiate into neurons and glial cells. It has been recently reported that GD3, a b-series ganglioside, is a marker molecule for identifying and isolating mouse NSCs. However, the expression of gangliosides in human NSCs is largely unknown. In the present study, we analysed the expression of gangliosides, GD2 and GD3, in human NSCs that were isolated from human brains at gestational week 17 in the form of neurospheres, which are floating clonal aggregates formed by NSCs in vitro. Employing immunocytochemistry, we found that human NSCs were strongly reactive to anti-GD2 antibody and relatively weakly reactive to anti-GD3 antibody. Treatment of these cells with an organic solvent such as 100% methanol, which selectively removes glycolipids from plasma membrane, abolished the immunoreactivity with those antibodies, indicating that the reactivity was due to GD2 and GD3, but not to GD2-/GD3-like glycoproteins or proteoglycans. The immunoreactivity of human NSCs to antibody against SSEA-1 (stage-specific embryonic antigen-1), a well-known carbohydrate antigen of NSCs, was not decreased by the treatment with 100% methanol, indicating that SSEA-1 is mainly carried by glycoproteins and/or proteoglycans in human NSCs. Our study suggests that GD2 and GD3 can be marker gangliosides for identifying human NSCs.     

Nogo—p4与NgR结合抑制神经干细胞分化为双极形星形胶质细胞的突起生长

目的观察Nogo—p4是否通过与NgR结合的途径对大鼠脊髓来源神经干细胞分化形成双极形星形胶质细胞突起长度产生抑制。方法取4只出生24h内的Wistar大鼠,悬浮培养法培养大鼠脊髓来源的神经干细胞。把神经干细胞分为A、B、C、D四组,A组加入血清,B组加入血清和Nogo—p4,C组神经干细胞经RNA干扰沉默NgR基因后加入血清分化,D组神经干细胞经RNA干扰沉默NgR基因后加入血清和Nogo—p4。分化第7d,GFAP抗体标记星形胶质细胞,使用Image—ProPlus5．0软件测量双极形星形胶质细胞突起长度。结果神经干细胞分化第7d,四组均可形成双极形星形胶质细胞。B组中双极形星形胶质细胞的突起长度明显短于其它各组。A、C、D组中双极形星形胶质细胞的突起长度没有显著差异。结论Nogo—p4经与NgR结合途径显著抑制脊髓来源神经干细胞分化成的双极形星形胶质细胞的突起生长。     

Neural stem cells producing an inducible and soluble form of Gas1 target and inhibit intracranial glioma growth

Background aimsGlioblastoma multiforme (GBM) is the most common and lethal primary brain tumor and current treatments have not improved its prognosis. Therefore, new strategies and therapeutic agents should be investigated. Growth arrest specific-1 (Gas1) is a protein that induces cell arrest and apoptosis of gliomas and a soluble form, tGas1, increases these effects acting in both autocrine and paracrine manners. Moreover, neural stem cells (NSCs) can be used as a vehicle to transport therapeutic molecules because they have innate tropism towards tumors.MethodsLentiviral vectors were used to obtain NSCs capable of expressing tGas1 in a regulated manner. The ability of engineered NSCs to track and reach GBM in vivo, produce tGas1, and their efficacy decreasing tumor growth and increasing the overall health and survival time of nude mice implanted with GBM were assessed.ResultsThe overexpression of tGas1 from NSCs decreased viability and induced cell arrest and apoptosis of GBM cells and also, albeit in a reduced manner, of NSCs themselves. NSCs migrate from one cerebral hemisphere to the contralateral, reach GBM, express the tGas1 transgene when induced by tetracycline and produce the protein. Tumor volume decreased by 77% compared with controls, and tGas1 improved the overall health and increased the survival time of mice implanted with GBM by 75%.ConclusionsWe demonstrated that tGas1 has an antineoplastic effect, and the results support the potential of tGas1 as an adjuvant for the treatment of gliomas.     

Effect and mechanism of mGluR6 on the biological function of rat embryonic neural stem cells

Here, we investigated the effects and molecular mechanisms of metabotropic glutamate receptor 6 (mGluR6) on rat embryonic neural stem cells (NSCs). Overexpression of mGluR6 significantly promoted the proliferation of NSCs and increased the diameter of neutrospheres after treatment for 24 h, 48 h and 72 h. Overexpression of mGluR6 promoted G1 to S phase transition, with significantly decreased cell ratio in G1/G0 phase but significantly increased cell ratio in S phase. Additionally, mGluR6 overexpression for 48 h decreased the early and late apoptosis significantly. Moreover, overexpression of mGluR6 significantly increased the expression of p-ERK1/2, Cyclin D1 and CDK2, while the expression of p-p38 was significantly decreased. On the contrary, these effects of mGluR6 overexpression were reversed by mGluR6 knockdown. In conclusion, mGluR6 promotes the proliferation of NSCs by activation of ERK1/2-Cyclin D1/CDK2 signaling pathway and inhibits the apoptosis of NSCs by blockage of the p38 MAPK signaling pathway.     

Muscarinic acetylcholine receptors involved in the regulation of neural stem cell proliferation and differentiation in vitro

Neural stem cells (NSCs) are currently considered powerful candidates for cell therapy in neurodegenerative disorders such as Parkinson's disease. However, it is not known when and how NSCs begin to differentiate functionally. Recent reports suggest that classical neurotransmitters such as acetylcholine (Ach) are involved in the proliferation and differentiation of neural progenitor cells, suggesting that neurotransmitters play an important regulatory role in development of the central nervous system (CNS). We have shown by calcium imaging and immunochemistry that proliferation and differentiation are enhanced by M2 muscarinic Ach receptors (mAchR) expressed on the NSC surface and on their neural progeny. Moreover, atropine, an mAchR antagonist, blocks the enhancement and inhibits the subsequent differentiation of NSCs. Further understanding of this neural-nutrition role of Ach might elucidate fetal brain development, the brain's response to injury, and learning and memory.     

胚胎神经干细胞移植及胶质细胞源性神经营养因子对大鼠脊髓损伤的修复作用

将胚胎神经干细胞(neural stem cells,NSCs)移植至成年大鼠损伤的脊髓,观察移植后NSCs的存活、迁移以及损伤后的功能恢复。实验结果显示：动物NSCs移植4周后,斜板实验平均角度和运动评分结果比对照组均有明显增高(P＜0．05),而脊髓损伤(spinal cord injury,SCI)处的空洞面积显著减小(P＜0．05);在NSCs中加入胶质细胞源性的神经营养因子(glial cell line-derived neurotrophic factor,GDNF)后,上述改变更加显著。移植后的NSCs不仅能存活,而且向损伤的头端和尾端迁移达3mm之远。这些结果表明,移植的NSCs不仅可以存活、迁移,还可减小SCI空洞面积,促进动物神经功能的恢复;此外,我们的结果还表明GDNF对SCI功能恢复有促进作用。