胞质分裂作用因子4过表达慢病毒载体的构建和稳定转染Neuro-2a细胞的建立

目的:构建胞质分裂作用因子4(DOCK4)过表达慢病毒载体,建立DOCK4稳定过表达的Neuro-2a细胞。方法:在美国国家生物信息中心(NCBI)查找DOCK4的序列并设计合成引物,采用聚合酶链式反应(PCR)法扩增获取DOCK4基因序列,通过Bam HⅠ和AgeⅠ限制性内切酶酶切后,将其与酶切后的慢病毒载体GV492进行连接,构建GV492-DOCK4过表达重组质粒,PCR法鉴定筛选出与目的基因片段长度大小相近的阳性克隆。将GV492-对照质粒和GV492-DOCK4过表达重组质粒分别转染至HEK293T细胞中,转染48 h后收集慢病毒进行包装并测定病毒滴度。将Neuro-2a细胞分为GV492-对照组和GV492-DOCK4组,分别采用GV492-对照组慢病毒和GV492-DOCK4过表达慢病毒感染Neuro-2a细胞,慢病毒感染复数(MOI)为100,感染72 h后采用嘌呤霉素(10 mg·L^(-1))筛选出成功感染GV492-对照组慢病毒和GV492-DOCK4过表达慢病毒的Neuro-2a细胞,荧光显微镜观察各组Neuro-2a细胞生长状态及绿色荧光蛋白表达情况;采用实时荧光定量PCR(RT-qPCR)法和Western blotting法检测各组Neuro-2a细胞中DOCK4 mRNA和DOCK4蛋白表达水平。结果:PCR检测,GV492-DOCK4过表达重组质粒的基因片段长度约为691 bp,测序结果显示GV492-DOCK4过表达重组质粒基因序列与设计合成的DOCK4过表达序列一致;GV492-对照组和GV492-DOCK4过表达组慢病毒的滴度分别为2.5×10^(8) TU·mL^(-1)和2.5×10^(8) TU·mL^(-1);荧光显微镜观察,各组Neuro-2a细胞生长状态良好且存在绿色荧光蛋白表达;RT-qPCR法检测,与GV492-对照组比较,GV492-DOCK4组Neuro-2a细胞中DOCK4 mRNA表达水平明显升高(P<0.01);Western blotting法检测,各组细胞在相对分子质量225000附近出现特异性条带,与GV492-对照组比较,GV492-DOCK4组Neuro-2a细胞中DOCK4蛋白表达水平明显升高(P<0.01)。结论:本研究成功构建DOCK4过表达慢病毒载体,建立了稳定过表达DOCK4的Neuro-2a细胞。

A Neuro T-Norm Fuzzy Logic Based System

In this study, we are first examining well-known approach to improve fuzzy reasoning model (FRM) by use of the genetic-based learning mechanism [1]. Later we propose our alternative way to build FRM, which has significant precision advantages and does not require any adjustment/learning. We put together neuro-fuzzy system (NFS) to connect the set of exemplar input feature vectors (FV) with associated output label (target), both represented by their membership functions (MF). Next unknown FV would be classified by getting upper value of current output MF. After that the fuzzy truths for all MF upper values are maximized and the label of the winner is considered as the class of the input FV. We use the knowledge in the exemplar-label pairs directly with no training. It sets up automatically and then classifies all input FV from the same population as the exemplar FVs. We show that our approach statistically is almost twice as accurate, as well-known genetic-based learning mechanism FRM.

沉默TRPM7对无镁外液致痫Neuro-2a细胞炎症反应的影响

目的观察沉默瞬时受体电位M7通道(transient receptor potential melastatin 7,TRPM7)对无镁外液致痫小鼠脑神经瘤Neuro-2a细胞炎症反应的影响。方法Neuro-2a细胞经脂质体转染TRPM7 siRNA,经无镁外液培养3 h建立癫痫细胞模型。实验分为4组:对照组(Control)、癫痫组(EP)、癫痫转染组(EP+si-TRPM7)和癫痫转染阴性对照组(EP+si-NC)。成模后24 h,利用实时荧光定量PCR技术检测TRPM7 mRNA表达;利用Western Blot检测HMGB1和TLR4蛋白的表达;利用ELISA方法检测上清液中TNF-α、IL-1β和IL-6的含量;CCK-8法检测细胞活力。结果成模后24 h,与Control组比较,EP组TRPM7 mRNA、HMGB1和TLR4蛋白表达增多,上清液中TNF-α、IL-1β和IL-6含量增多,细胞活力降低。与EP+si-NC组比较,EP+si-TRPM7组TRPM7 mRNA、HMGB1和TLR4蛋白表达减少,上清液中TNF-α、IL-1β和IL-6含量减少,细胞活力增高(P<0.01)。结论沉默TRPM7能抑制HMGB1/TLR4通路,减轻炎症反应,对无镁外液致痫细胞有保护作用。

50 Hz磁场暴露对Neuro2a/APP(695)细胞基因转录的影响

目的研究50 Hz磁场暴露对Neuro2a/APP(695)细胞基因转录的影响。方法Neuro2a/APP(695)细胞简单随机分为假性辐照组和磁场暴露组(n=3)。暴露条件为1.0 mT 50 Hz正旋波磁场,4 h/d,连续3 d;假性辐照组细胞除无磁场暴露外,余同磁场暴露组。暴露结束后按标准方法送样,进行转录组测序检测,包括样品RNA提取、数据质量评价和数据分析等。结果50 Hz磁场暴露后Neuro2a/APP(695)细胞有141种定性的基因表达发生了明显的变化,其中有129种表达上调、12种表达下调。GO富集分析结果显示,Neuro2a/APP(695)细胞中62种上调差异表达基因涉及432类显著GO功能富集,其中涉及生物学过程337类、细胞组分16类、分子功能79类;3种下调差异表达基因共涉及275类显著GO功能富集,其中涉及生物学过程260类、细胞组分5类、分子功能10类。KEGG通路分析显示,这些差异基因可能参与了20条KEGG通路,其中2个下调差异表达基因通路,18个上调差异表达基因通路。结论50 Hz磁场暴露可能对Neuro2a/APP(695)细胞的黏附连接、Hippo信号通路、糖胺聚糖生物合成-硫酸软骨素/硫酸皮肤素、蛋白消化和吸收和甘露糖型O-聚糖生物合成等方面产生影响,以上通路可能是50 Hz磁场对Neuro2a/APP(695)细胞产生影响的主要途径。

Neuro-meningeal Tuberculosis in Adult Senegalese Patients: Profile and Outcome of Cases Diagnosed at a Referral Service, from 2015 to 2020

Background: Among patients treated for tuberculosis, 2% to 5% have a Central Nervous System (CNS) lesion, and its frequency rises to 10% in HIV-infected patients. Neuro-meningeal tuberculosis (NMT) is responsible for death and severe permanent neurological damage. This poor prognosis requires early diagnosis and rapid initiation of specific treatment. Unfortunately, the great clinical polymorphism and the lack of specificity of radiological and biological signs are frequently responsible for a delay in diagnosis and management. Senegal is one of the African countries where tuberculosis has remained a concern until now. And there are no studies carried out on this subject. Objective: The objective of this study was to describe the profile and outcome of Neuro-meningeal tuberculosis (NMT) cases diagnosed at the infectious diseases department (SMIT) of Fann University Hospital in Dakar, (referral service for management of tuberculosis). Methods: We carried out a retrospective, descriptive and analytical study, reviewing medical records of adults diagnosed with NMT at the SMIT of Fann Hospital from January 2015 to December 2020. Results: We collected 55 cases of NMT. The median age was 38 years [range 16 - 77 years]. The sex ratio (M/F) was 3.23. HIV patients represented 41.82% of cases. A history of tuberculosis was found in 25.5% of cases. The delay in consultation was greater than one month in 60% of patients. Headaches were the most constant reason for consultation (94.55%). Meningeal signs were present in 94.55% of patients, and consciousness disorders and intracranial hypertension were present in 63.64% and 56.36% respectively. Nerve palsy was found in 38.18%. CSF was clear in 81.64%. GeneXpert MTB/RIF in CSF was performed in 33 patients and was positive in 4 patients. Brain CT was abnormal in 72.09% of cases. Tuberculoma, hydrocephalus and meningeal contrast enhancement were the main lesions. The neuro-meningeal localization was associated with a pulmonary form in 32.7%. The lethality rate was 21.8%;higher in women (46.2% vs 14.3%;p = 0.01), in patients with a delay in consultation > 1 month (p = 0.03), and in patients who presented with consciousness disorders (p = 0.007). Conclusion: Despite the availability of the GeneXpert MTB/RIF, diagnosis of NMT remains difficult. Because of its variable clinical expression and the low sensitivity of the GeneXpert MTB/rif in the CSF, it exposes patients to serious complications. Among the factors associated with death, we found consciousness disorders, a long delay in diagnosis.

Effects of microcystin-LR on hippocampal N-acetylaspartate and neurobehaviors in rats

The effects of low-doses of microcystin-leucinearginine （ MC-LR ） exposure on neurobehaviors and N-acetylaspartate （NAA） expression in the hippocampus of rats were investigated. After male Sprague-Dawley （SD） rats were treated intra-gastrically with different doses of MC-LR for 90 d, the locomotor activity, spatial learning and memory function were evaluated in the rats after treatment using open field tests and Morris water maze tests. The results show that MC-LR exposure can lead to impairment of the spatial learning capacity and locomotor activity in rats at the dose of 2. 00 p,g/kg. The levels of NAA in the hippocampus were measured by magnetic resonance spectroscopy （MRI）. A significant decrease of NAA/Cr ratio （ P 〈 0. 05） was observed in the hippocampous. This study indicates that intra-gastrical exposure to low-doses of MC-LR has adverse effects on neuronal behavior and NAA levels in the hippocampous.

Transcription factor-based gene therapy to treat glioblastoma through direct neuronal conversion

Objective:Glioblastoma(GBM)is the most prevalent and aggressive adult primary cancer in the central nervous system.Therapeutic approaches for GBM treatment are under intense investigation,including the use of emerging immunotherapies.Here,we propose an alternative approach to treat GBM through reprogramming proliferative GBM cells into non-proliferative neurons.Methods:Retroviruses were used to target highly proliferative human GBM cells through overexpression of neural transcription factors.Immunostaining,electrophysiological recording,and bulk RNA-seq were performed to investigate the mechanisms underlying the neuronal conversion of human GBM cells.An in vivo intracranial xenograft mouse model was used to examine the neuronal conversion of human GBM cells.Results:We report efficient neuronal conversion from human GBM cells by overexpressing single neural transcription factor Neurogenic differentiation 1(Neuro D1),Neurogenin-2(Neurog2),or Achaete-scute homolog 1(Ascl1).Subtype characterization showed that the majority of Neurog2-and Neuro D1-converted neurons were glutamatergic,while Ascl1 favored GABAergic neuron generation.The GBM cell-converted neurons not only showed pan-neuronal markers but also exhibited neuron-specific electrophysiological activities.Transcriptome analyses revealed that neuronal genes were activated in glioma cells after overexpression of neural transcription factors,and different signaling pathways were activated by different neural transcription factors.Importantly,the neuronal conversion of GBM cells was accompanied by significant inhibition of GBM cell proliferation in both in vitro and in vivo models.Conclusions:These results suggest that GBM cells can be reprogrammed into different subtypes of neurons,leading to a potential alternative approach to treat brain tumors using in vivo cell conversion technology.

Neuro-rejuvenation for neuronal function

Neurodegenerative eye diseases, such as glaucoma, cause irreversible vision loss in millions of patients worldwide, creating serious medical, economic and social issues. Like other mammalian central nervous system tracts, optic nerve intrinsically lacks the capacity for axonal growth and its surrounding environment is also non-permissive to regeneration. Any axonal damage also triggers a vicious cycle of retinal ganglion cell （RGC） death. Exploring methods that can enhance RGCs survival and promote axonal regeneration will not only enable vision restoration for millions of patients, but also shed light on the treatment of other neurodegenerative diseases. In this review article, we will go through three current approaches to cure neu- rodegenerative eye diseases, including cell based therapy, neuro-regeneration and neuro-rejuvenation.

黄芩苷对Neuro2A细胞氧糖剥夺的保护作用

目的观察黄芩苷对体外培养小鼠神经母细胞瘤Neuro2A细胞株氧糖剥夺所致损伤的保护作用。方法利用体外培养的Neuro2A细胞,通过去除培养液中的糖和氧气来模拟脑缺血缺氧,用不同浓度的黄芩苷作用于Neuro2A细胞,应用Annexin V-FITC/PI染色,流式细胞术检测细胞凋亡,应用四唑盐(MTT)法检测细胞的活性。结果黄芩苷在6.25,12.5,25μmol.L-1的浓度范围之内,可对缺血缺氧Neuro2A细胞起到保护作用,主要是减少细胞早期凋亡。结论在一定浓度范围之内黄芩苷可保护缺血缺氧Neuro2A细胞,提示对缺血性脑损伤有保护作用,值得进一步研究。

垂体腺苷环化酶激活多肽抑制β淀粉样蛋白对Neuro-2a细胞神经毒性作用的机制

通过MTT方法检测细胞活性 ,同时采用激光共聚焦显微镜技术检测细胞内游离钙离子的瞬时运动 ,研究了垂体腺苷环化酶激活多肽 (pituitaryadenylatecyclaseactivatingpolypeptide 2 7,PACAP2 7)通过调节细胞内钙对抗淀粉样蛋白Aβ2 5 35引起Neuro 2a细胞神经毒性作用的可能机制。结果表明 ,PACAP在一定浓度范围内 (<0 1μmol/L)可提高Neuro 2a细胞增殖能力并对抗Aβ引起的神经毒性 ,此作用可以被PACAP受体竞争性拮抗剂PACAP6 2 7所抑制。 2 5 μmol/LAβ使细胞内钙离子缓慢上升 ,并有一个较长时间的平台期。 0 1μmol/L的PACAP使细胞内钙离子迅速升高后下降 ,10min后回到接近基线水平 ,伴有较长时间的不应期。用PACAP预处理细胞 10min后Aβ引起细胞内钙的慢上升不再出现。推测 ,PACAP受体激活引起瞬时内向钙离子运动 ,而后伴随一个较长时间的不应期 ,可能是一个消除凋亡或阻止凋亡启动的保护机制。

血清型A肉毒杆菌神经毒素重链对Neuro-2a细胞的促神经突起再生作用

目的:观察血清型A肉毒杆菌神经毒素重链(botulinum neurotoxin serotype A heavy chain,Bo NT/A HC)对Neuro-2a细胞的促神经突起再生作用并探讨与其相关的细胞内信号机制。方法:采用体外细胞培养技术,在培养液中加入不同浓度的Bo NT/A HC(0.01 nmol/L、0.1 nmol/L、1 nmol/L和10 nmol/L)进行干预,于24 h、48 h和72 h时收集细胞进行免疫荧光染色,再计算细胞突起长度及有突起细胞的百分比;在此基础上,选择最有效的Bo NT/A HC浓度作为处理剂量加入细胞培养液,于Bo NT/A HC作用后不同时点收集全细胞蛋白,采用Western blot检测p-ERK1/2及p-Akt的蛋白水平。结果:当Bo NT/A HC浓度为0.1 nmol/L、1 nmol/L和10 nmol/L时,细胞突起的长度及有突起细胞的百分比与对照组相比皆明显增加,差异显著(P<0.05),其中1 nmol/L效果最显著。在细胞培养液内加入1 nmol/L Bo NT/A HC后,p-ERK1/2的蛋白水平呈增加趋势,其中Bo NT/A HC作用60 min后,p-ERK1/2的增加与对照组相比差异显著(P<0.05);与p-ERK1/2变化趋势类似,细胞培养液内加入1 nmol/L的Bo NT/A HC后,p-Akt的蛋白水平也呈增加趋势,其中Bo NT/A HC作用15 min和60 min时,p-Akt增加显著(P<0.05)。结论:一定剂量的Bo NT/A HC可以促进神经细胞突起再生和生长;Bo NT/A HC对Neuro-2a细胞的促神经突起再生作用机制可能通过激活与神经再生相关的信号蛋白ERK1/2和Akt的磷酸化而实现。

miRNA-99a对过氧化氢诱导neuro-2a细胞氧化损伤的影响

目的研究microRNA-99a(miR-99a)对过氧化氢所诱导神经细胞neuro-2a氧化损伤的影响。方法常规培养neuro-2a细胞并分为3组:正常对照组,过氧化氢100μmol/L刺激组,miR-99a预处理组(转染miRNA-99a mimics+过氧化氢100μmol/L刺激),用CCK-8试剂盒检测细胞存活率,生化试剂盒检测还原型烟酰胺腺嘌呤二核苷酸(nicotinamide adenine dinucleotide,NADH)含量和总超氧化物歧化酶(total superoxide dismutase,T-SOD)、锰超氧化物歧化酶(manganese superoxide dismutase,MnSOD)活性,Western blotting检测突触小体相关蛋白(synaptosoma associated protein of molecular mass 25 000,SNAP25)及Mn-SOD、细胞外超氧化物歧化酶(extracellular SOD,EC-SOD)的蛋白表达水平。结果与正常对照组相比,过氧化氢刺激的2组细胞存活率明显下降,分别为85%和89%(P<0.05),但miR-99a预处理组的细胞存活率下降程度较小仅为11%(P<0.05)。进一步研究发现,过氧化氢刺激引起细胞T-SOD、Mn-SOD活性降低(P<0.05),转染miR-99a mimics不但能增强T-SOD和Mn-SOD的活性,还能促进Mn-SOD和EC-SOD的表达(P<0.05)。过氧化氢导致细胞中NADH含量降低(P<0.05),miR-99a能够增加NADH含量甚至高于正常细胞水平(P<0.05)。miR-99a还有增加neuro-2a细胞表达SNAP25的趋势。结论 miR-99a对过氧化氢诱导neuro-2a细胞引起的氧化损伤具有保护作用。

Primary large cell neuroendocrine carcinoma in the common bile duct:First Asian case report

Large cell neuroendocrine carcinoma (LCNEC) in the biliary system is a poorly differentiated, high-grade neuroendocrine tumor. These tumors exhibit aggressive behavior and an increased tendency for early nodal and distant metastases. Herein, we report an unusual case of a pure primary LCNEC of the common bile duct (CBD). A 75-year-old female presented with nausea and jaundice. The patient underwent a CBD excision with lymph node dissection. Upon histological and immunohistochemical examination, the tumor exhibited pure large cell-type neuroendocrine features. Metastases were noted in two of the eight lymph nodes. The patient was administered adjuvant chemotherapy. The patient&#x02019;s cancer recurred 7 mo after surgery, and the patient died from liver failure 5 mo after recurrence. The prognosis of LCNEC of CBD remains poor despite curative resection and adjuvant chemotherapy. The role of additional therapies, such as multimodal treatment including radiation therapy, must be further studied to improve the prognoses of patients.

Neuro-2a细胞替代神经元原代培养进行神经轴突测量实验研究

目的建立使用小鼠神经母细胞瘤Neuro-2a细胞替代原代培养神经元进行神经轴突测量的方法,用于神经损伤研究。方法使用浓度200μmol/L、500μmol/L、1 000μmol/L过氧化氢处理Neuro-2a细胞12h,戊二醛固定,生物染色,在光学显微镜下手动测量突起长度。结果过氧化氢可剂量依赖性引起神经突起逐渐回缩变短,1 000μmol/L过氧化氢处理组光镜下见不到明显突起,突起测量数据显示,过氧化氢处理后突起长度与未经处理细胞有显著差异。结论 Neuro-2a细胞在一定程度上可替代原代培养神经元进行轴突测量研究,该测量方法可用于神经轴突再生研究。

Activin A maintains cerebral cortex neuronal survival and increases voltage-gated Na^+ neuronal current

Activin A, which was first described in 1986, has been shown to maintain hippocampal neuronal survival. Activin A increases intracellular free Ca2＋ via L-type Ca2＋ channels. Our previous study showed that activin A promotes neurite growth of dorsal root ganglia in embryonic chickens and inhibits nitric oxide secretion. The present study demonstrated for the first time that activin A could maintain cerebral cortex neuronal survival in vitro for a long period, and that activin A was shown to increase voltage-gated Na＋ current （/Na） in Neuro-2a cells, which was recorded by patch clamp technique. The present study revealed a novel mechanism for activin A, as well as the influence of activin A on neurons by regulating expressions of vasoactive intestine peptide and inducible nitric oxide synthase.

Role of miR-124 in the regulation of retinoic acid-induced Neuro-2A cell differentiation

Retinoic acid can cause many types of cells,including mouse neuroblastoma Neuro-2 A cells,to differentiate into neurons.However,it is still unknown whether microRNAs(miRNAs)play a role in this neuronal differentiation.To address this issue,real-time polymerase chain reaction assays were used to detect the expression of several differentiation-related miRNAs during the differentiation of retinoic acid-treated Neuro-2 A cells.The results revealed that miR-124 and miR-9 were upregulated,while miR-125 b was downregulated in retinoic acid-treated Neuro-2 A cells.To identify the miRNA that may play a key role,miR-124 expression was regulated by transfection of miRNA mimics or inhibitors.Morphological analysis results showed that inhibition of miR-124 expression reversed the effects of retinoic acid on neurite outgrowth.Moreover,miR-124 overexpression alone caused Neuro-2 A cells to differentiate into neurons,and its inhibitor could block this effect.These results suggest that miR-124 plays an important role in retinoic acid-induced differentiation of Neuro-2 A cells.

Neuroprotective effect of panax notoginseng saponins and its main components

Stroke is the third leading cause of death and the first cause of adult disability in industrial countries [1]. It is charicaterized by hemiplegia, hemianopsia, aphasia, mouth askew and sever sequelae. It is considered that an ischemic disease without any specific treatment method and few effective drugs such as tPA (human tissue-type plasminogen activator) and Edarovone with specific therapeutic window will cause a lot of disadvantages if being used inaccurate. Root of Panax notoginseng (PN) which is one of traditional Chinese medicines (TCMs), was first found in “Shennong’s Classic of Materia Medica” around 200 AD. Panax notogineng saponins(PNS) is a multi-components mixture containing ginseng and saponins as the most important bioactive components which are commonly used in clinical treatment. Also, ginseng and saponins form the main components of many herbal medicines in the market, e.g., Xueshuantong injection [2], Xuesaitong injection [3], Xuesaitong soft capsule [4] and so on. The main monomers of Panax notoginseng saponins (PNS) are Ginsenoside-Rb1, Gensenoside-Rg1, Gensenoside-Re, Gensenoside-Rd and Panax notoginseng saponins-R1 [5]. In this review, we found some important points as well as shortcomings that require special consideration. We therefore highlighted the advances in neuro-protection of PNS and its main monomers in the area of experimental research.

酒精对小鼠脑神经瘤细胞Neuro2a增殖的影响

目的探讨酒精通过控制中心体增长影响小鼠脑神经瘤细胞Neuro2a增殖的机制。方法免疫荧光细胞计数检测酒精对细胞周期进程的改变;免疫荧光法检测酒精对纺锤体表型以及对外源性和内源性中心体蛋白P4.1相关蛋白(CPAP)中心体定位浓度的影响。结果 100 mmol/L酒精处理Neuro2a细胞96 h后,阻碍了细胞周期的进程,减少了进入有丝分裂期的细胞量;有丝分裂期纺锤体的表型出现多种异常;酒精通过降低中心体上内源性和外源性CPAP的定位浓度,抑制了中心体的增长。结论酒精抑制CPAP在中心体增长中的功能,导致有丝分裂期纺锤体排列异常,从而阻止细胞进入有丝分裂期,引起Neuro2a细胞数量减少。

miR-16促进Neuro2a细胞的凋亡

目的检测过表达miR-16对小鼠Neuro2a细胞周期和凋亡的影响,探讨miR-16在肿瘤发病过程中的可能机制。方法 构建能够在细胞中过表达miR-16的真核表达载体pcDNA3.1-miR-16,利用Real-time PCR验证了表达载体的过表达效应。应用pcDNA3.1-miR-16载体转染Neuro2a细胞,利用流式细胞术和TUNEL法检测Neuro2a细胞周期及凋亡改变情况。结果 转染过表达pcDNA3.1-miR-16载体后,成熟的miR-16表达与对照组相比明显升高(P<0.05)。在Neuro2a细胞中过表达miR-16后,用流式细胞术检测发现,Neuro2a细胞周期未见明显改变,与对照组相比,凋亡细胞数量有显著增加;进一步通过TUNEL法验证,发现miR-16的过表达能够促进Neuro2a的细胞凋亡。结论 过表达miR-16能够显著促进Neuro2a细胞凋亡而对细胞周期并无影响,提示miR-16可能对肿瘤治疗起作用。

激活素A对Neuro-2a细胞电压门控钠电流的作用

目的:研究激活素A(activinA)对Neuro-2a细胞电压门控钠电流(INa)的作用及其机制,为激活素A在神经系统疾病中的应用奠定基础。方法:培养小鼠源性Neuro-2a细胞,分为IgG对照组和抗激活素受体ⅡA(ActRⅡA)抗体染色组,免疫组织化学染色观察ActRⅡA在Neuro-2a细胞中是否表达;将Neuro-2a细胞随机分为正常对照组和激活素A组,采用全细胞膜片钳技术检测激活素A对Neuro-2a细胞INa的作用;采用RT-PCR检测激活素A对血管活性肠肽(VIP)及诱导型一氧化氮合酶(iNOS)mRNA表达的影响。结果:正常Neuro-2a细胞中可检测到ActRⅡA的表达;与正常对照组比较,激活素A明显增加Neuro-2a细胞INa(P<0.05);激活素A组Neuro-2a细胞VIPmRNA表达明显高于正常对照组(P<0.05),而iNOSmRNA表达低于正常对照组(P<0.05)。结论:激活素A具有增加Neuro-2a细胞电压门控Na+电流的作用,VIP和iNOS途径可能参与了激活素A调控神经细胞的功能。