Neuroprotective effect of LSS on Aβ_(1-42)-induced BV-2 microglial cells through the inhibition of neuroinflammation

OBJECTIVE To investigate the effect of neuroprotective effect of lychee seed saponins(LSS) in BV-2.METHODS Aβ_(1-42) induced BV-2 cells were incubated with LSS for 12 h,the content of the inflammatory factors such as IL^(-1)β,TNF-α,COX-2 and i NOS in the supernatant of BV-2 cell were measured by ELISA.The detection of the m RNA levels and the protein expression of the inflammatory factors including IL^(-1)β,TNF-α,COX-2 and i NOS using real-time PCR and Western blotting,respectively.RESULTS The level of IL^(-1)β,COX-2 and i NOS significantly increased with the treatment of Aβ_(1-42),and 0.117 mg·L^(-1)-0.469 mg·L^(-1) LSS can inhibit these increased level.CONCLUSION LSS conferred neuroprotection via inhibiting the inflammatory factors expression.

Inhibiting SHP2 reduces glycolysis, promotes microglial M1 polarization, and alleviates secondary inflammation following spinal cord injury in a mouse model

Reducing the secondary inflammatory response, which is partly mediated by microglia, is a key focus in the treatment of spinal cord injury. Src homology 2-containing protein tyrosine phosphatase 2(SHP2), encoded by PTPN11, is widely expressed in the human body and plays a role in inflammation through various mechanisms. Therefore, SHP2 is considered a potential target for the treatment of inflammation-related diseases. However, its role in secondary inflammation after spinal cord injury remains unclear. In this study, SHP2 was found to be abundantly expressed in microglia at the site of spinal cord injury. Inhibition of SHP2 expression using siRNA and SHP2 inhibitors attenuated the microglial inflammatory response in an in vitro lipopolysaccharide-induced model of inflammation. Notably, after treatment with SHP2 inhibitors, mice with spinal cord injury exhibited significantly improved hind limb locomotor function and reduced residual urine volume in the bladder. Subsequent in vitro experiments showed that, in microglia stimulated with lipopolysaccharide, inhibiting SHP2 expression promoted M2 polarization and inhibited M1 polarization. Finally, a co-culture experiment was conducted to assess the effect of microglia treated with SHP2 inhibitors on neuronal cells. The results demonstrated that inflammatory factors produced by microglia promoted neuronal apoptosis, while inhibiting SHP2 expression mitigated these effects. Collectively, our findings suggest that SHP2 enhances secondary inflammation and neuronal damage subsequent to spinal cord injury by modulating microglial phenotype. Therefore, inhibiting SHP2 alleviates the inflammatory response in mice with spinal cord injury and promotes functional recovery postinjury.

Recombinant chitinase-3-like protein 1 alleviates learning and memory impairments via M2 microglia polarization in postoperative cognitive dysfunction mice

Postoperative cognitive dysfunction is a seve re complication of the central nervous system that occurs after anesthesia and surgery,and has received attention for its high incidence and effect on the quality of life of patients.To date,there are no viable treatment options for postoperative cognitive dysfunction.The identification of postoperative cognitive dysfunction hub genes could provide new research directions and therapeutic targets for future research.To identify the signaling mechanisms contributing to postoperative cognitive dysfunction,we first conducted Gene Ontology and Kyoto Encyclopedia of Genes and Genomes pathway enrichment analyses of the Gene Expression Omnibus GSE95426 dataset,which consists of mRNAs and long non-coding RNAs differentially expressed in mouse hippocampus3 days after tibial fracture.The dataset was enriched in genes associated with the biological process"regulation of immune cells,"of which Chill was identified as a hub gene.Therefore,we investigated the contribution of chitinase-3-like protein 1 protein expression changes to postoperative cognitive dysfunction in the mouse model of tibial fractu re surgery.Mice were intraperitoneally injected with vehicle or recombinant chitinase-3-like protein 124 hours post-surgery,and the injection groups were compared with untreated control mice for learning and memory capacities using the Y-maze and fear conditioning tests.In addition,protein expression levels of proinflammatory factors(interleukin-1βand inducible nitric oxide synthase),M2-type macrophage markers(CD206 and arginase-1),and cognition-related proteins(brain-derived neurotropic factor and phosphorylated NMDA receptor subunit NR2B)were measured in hippocampus by western blotting.Treatment with recombinant chitinase-3-like protein 1 prevented surgery-induced cognitive impairment,downregulated interleukin-1βand nducible nitric oxide synthase expression,and upregulated CD206,arginase-1,pNR2B,and brain-derived neurotropic factor expression compared with vehicle treatment.Intraperitoneal administration of the specific ERK inhibitor PD98059 diminished the effects of recombinant chitinase-3-like protein 1.Collectively,our findings suggest that recombinant chitinase-3-like protein 1 ameliorates surgery-induced cognitive decline by attenuating neuroinflammation via M2 microglial polarization in the hippocampus.Therefore,recombinant chitinase-3-like protein1 may have therapeutic potential fo r postoperative cognitive dysfunction.

灯盏乙素通过环状GMP-AMP合酶-干扰素基因刺激因子通路抑制BV-2小胶质细胞介导的神经炎症

目的探讨灯盏乙素对脂多糖(LPS)诱导的BV-2小胶质细胞神经炎症的影响。方法培养BV-2小胶质细胞系,将BV-2小胶质细胞分为对照组(Ctrl)、环状GMP-AMP合酶(cGAS)抑制剂RU320521(RU.521)组、LPS组、LPS+RU.521组、LPS+灯盏乙素预处理(LPS+S)组、LPS+S+RU.521组,共6组。Western blotting及免疫荧光双标染色法检测并观察BV-2小胶质细胞中cGAS、干扰素基因刺激因子(STING)、核因子κB(NF-κB)、磷酸化NF-κB(p-NF-κB)、PYD结构域蛋白3(NLRP3)和肿瘤坏死因子α(TNF-α)的表达变化(n=3)。结果Western blotting和免疫荧光双标染色均显示,与对照组相比,LPS诱导后,BV-2小胶质细胞中cGAS、STING、p-NF-κB、NLRP3和TNF-α蛋白的表达水平显著升高(P<0.05);与LPS组相比,LPS+S组中cGAS、STING、p-NF-κB、NLRP3和TNF-α蛋白的表达水平显著下降(P<0.05)。使用cGAS通路抑制剂RU.521后显示了与灯盏乙素预处理组相似的作用效果。此外,NF-κB在各组的变化不明显(P>0.05)。结论灯盏乙素干预抑制BV-2小胶质细胞介导的神经炎症反应,可能与cGAS-STING信号通路有关。

Tamoxifen Induces Apoptosis of Mouse Microglia Cell Line BV-2 Cells via both Mitochondrial and Death Receptor Pathways

Little is known about whether tamoxifen (TAM) can affect resting state microglia apoptosis and about the cellular mechanism that may account for this. To explore this question, we incubated the microglia cell line BV-2 cells with TAM at different concentrations. Cell viability was assessed by the MTT assay, and flow cytometric analysis was performed to detect the cell apoptosis rate. Furthermore, mitochondrial membrane potential (Δψm) was tested by flow cytometry, and Bax, Bcl-2, Fas, and Fas-L expression was detected by Western blot. The results demonstrated that TAM decreased cell viability and induced apoptosis of BV-2 cells in a concentration- and time-dependent manner. In addition, disruption of Δψm was followed by up-regulated expression of pro-apoptotic Bax, Fas and Fas-L, and down-regulated expression of anti-apoptotic Bcl-2. These results indicate that TAM may induce apoptosis of BV-2 cells through both mitochondria- and death receptor-mediated pathways.

SphK2在氧糖剥夺/复糖复氧模型中对BV-2细胞损伤的影响

目的:观察BV-2小胶质细胞在氧糖剥夺/复糖复氧(OGD/R)中鞘氨醇激酶2(SphK2)的表达情况,并探讨SphK2是否参与了OGD/R致BV-2小胶质细胞的损伤过程。方法:采用小鼠BV-2小胶质细胞制备OGD/R模型,选取氧糖剥夺时间为2 h,复氧复糖时间为0 h,3 h,6 h,12 h,24 h。(1)设对照组,OGD 2 h组,OGD 2 h/R 3 h组,OGD 2 h/R 6 h组,OGD 2 h/R 12 h组,OGD 2 h/R 24 h组,观察细胞形态变化。细胞经OGD/R处理后CCK-8法检测细胞存活率。(2)设对照组,OGD 2 h/R 12 h组,OGD 2 h/R 12 h+ABC294640(SphK2特异抑制剂)组,用q-PCR及Western blot测定SphK2的基因及蛋白表达变化。结果:与对照组相比,随着OGD/R时间的延长,BV-2活力逐渐下降(P<0.001),细胞形态发生了不同程度的改变,且有不同程度的损伤;通过观察细胞生存情况确定OGD2 h/R12 h为最适宜的OGD/R时间,与对照组相比,经OGD/R处理后BV-2细胞中SphK2 mRNA表达水平显著升高(P<0.05),加入ABC294640显著抑制其表达升高(P<0.001);与对照组相比,经OGD/R处理后BV-2细胞中SphK2蛋白表达水平显著升高(P<0.001),加入ABC294640后,SphK2蛋白表达明显降低(P<0.001)。结论:OGD/R损伤后的小胶质细胞可以被SphK2激活,在其损伤过程中发挥着调控作用。

PrP 106-126 Altered PrP mRNA Gene Expression in Mouse Microglia BV-2 Cells

Prion diseases are infectious and fatal neurodegenerative diseases.The pathogenic agent is an abnormal prion protein aggregate.Microglial activation in the centre nervous system is a characteristic feature of prion disease.In this study,we examined the effect of PrP 106-126 on PrP mRNA gene expression in Mouse microglia cells BV-2 by real-time quantitative PCR.PrP mRNA expression level was found to be significantly increased after 18 h exposure of BV-2 cells to PrP 106-126,with 3-fold increase after 18 h and 4.5-fold increase after 24 h and BV-2 cells proliferating occurred correspondingly.Our results provide the first in vitro evidence of the increase of PrP mRNA levels in microglial cells exposed to PrP 106-126,and indicate that microglial cells might play a critical role in prion pathogenesis.

High-dose dexamethasone regulates microglial polarization via the GR/JAK1/STAT3 signaling pathway after traumatic brain injury

Although microglial polarization and neuroinflammation are crucial cellular responses after traumatic brain injury,the fundamental regulatory and functional mechanisms remain insufficiently understood.As potent anti-inflammato ry agents,the use of glucoco rticoids in traumatic brain injury is still controversial,and their regulatory effects on microglial polarization are not yet known.In the present study,we sought to determine whether exacerbation of traumatic brain injury caused by high-dose dexamethasone is related to its regulatory effects on microglial polarization and its mechanisms of action.In vitro cultured BV2 cells and primary microglia and a controlled cortical impact mouse model were used to investigate the effects of dexamethasone on microglial polarization.Lipopolysaccharide,dexamethasone,RU486(a glucocorticoid receptor antagonist),and ruxolitinib(a Janus kinase 1 antagonist)were administered.RNA-sequencing data obtained from a C57BL/6 mouse model of traumatic brain injury were used to identify potential targets of dexamethasone.The Morris water maze,quantitative reverse transcription-polymerase chain reaction,western blotting,immunofluorescence and confocal microscopy analysis,and TUNEL,Nissl,and Golgi staining were performed to investigate our hypothesis.High-throughput sequencing results showed that arginase 1,a marker of M2 microglia,was significantly downregulated in the dexamethasone group compared with the traumatic brain injury group at3 days post-traumatic brain injury.Thus dexamethasone inhibited M1 and M2 microglia,with a more pronounced inhibitory effect on M2microglia in vitro and in vivo.Glucocorticoid receptor plays an indispensable role in microglial polarization after dexamethasone treatment following traumatic brain injury.Additionally,glucocorticoid receptor activation increased the number of apoptotic cells and neuronal death,and also decreased the density of dendritic spines.A possible downstream receptor signaling mechanism is the GR/JAK1/STAT3 pathway.Overactivation of glucocorticoid receptor by high-dose dexamethasone reduced the expression of M2 microglia,which plays an antiinflammatory role.In contrast,inhibiting the activation of glucocorticoid receptor reduced the number of apoptotic glia and neurons and decreased the loss of dendritic spines after traumatic brain injury.Dexamethasone may exe rt its neurotoxic effects by inhibiting M2 microglia through the GR/JAK1/STAT3 signaling pathway.

C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 pathway as a therapeutic target and regulatory mechanism for spinal cord injury

Spinal cord injury involves non-reversible damage to the central nervous system that is characterized by limited regenerative capacity and secondary inflammatory damage.The expression of the C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 axis exhibits significant differences before and after injury.Recent studies have revealed that the C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 axis is closely associated with secondary inflammatory responses and the recruitment of immune cells following spinal cord injury,suggesting that this axis is a novel target and regulatory control point for treatment.This review comprehensively examines the therapeutic strategies targeting the C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 axis,along with the regenerative and repair mechanisms linking the axis to spinal cord injury.Additionally,we summarize the upstream and downstream inflammatory signaling pathways associated with spinal cord injury and the C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 axis.This review primarily elaborates on therapeutic strategies that target the C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 axis and the latest progress of research on antagonistic drugs,along with the approaches used to exploit new therapeutic targets within the C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 axis and the development of targeted drugs.Nevertheless,there are presently no clinical studies relating to spinal cord injury that are focusing on the C-C motif chemokine ligand 2/C-C motif chemokine receptor 2 axis.This review aims to provide new ideas and therapeutic strategies for the future treatment of spinal cord injury.

Microglia:a promising therapeutic target in spinal cord injury

Microglia are present throughout the central nervous system and are vital in neural repair,nutrition,phagocytosis,immunological regulation,and maintaining neuronal function.In a healthy spinal cord,microglia are accountable for immune surveillance,however,when a spinal cord injury occurs,the microenvironment drastically changes,leading to glial scars and failed axonal regeneration.In this context,microglia vary their gene and protein expression during activation,and proliferation in reaction to the injury,influencing injury responses both favorably and unfavorably.A dynamic and multifaceted injury response is mediated by microglia,which interact directly with neurons,astrocytes,oligodendrocytes,and neural stem/progenitor cells.Despite a clear understanding of their essential nature and origin,the mechanisms of action and new functions of microglia in spinal cord injury require extensive research.This review summarizes current studies on microglial genesis,physiological function,and pathological state,highlights their crucial roles in spinal cord injury,and proposes microglia as a therapeutic target.

Inhibiting ceramide synthase 5 expression in microglia decreases neuroinflammation after spinal cord injury

Microglia,the resident monocyte of the central nervous system,play a crucial role in the response to spinal cord injury.However,the precise mechanism remains unclear.To investigate the molecular mechanisms by which microglia regulate the neuroinflammatory response to spinal cord injury,we performed single-cell RNA sequencing dataset analysis,focusing on changes in microglial subpopulations.We found that the MG1 subpopulation emerged in the acute/subacute phase of spinal cord injury and expressed genes related to cell pyroptosis,sphingomyelin metabolism,and neuroinflammation at high levels.Subsequently,we established a mouse model of contusive injury and performed intrathecal injection of siRNA and molecular inhibitors to validate the role of ceramide synthase 5 in the neuroinflammatory responses and pyroptosis after spinal cord injury.Finally,we established a PC12-BV2 cell co-culture system and found that ceramide synthase 5 and pyroptosis-associated proteins were highly expressed to induce the apoptosis of neuron cells.Inhibiting ceramide synthase 5 expression in a mouse model of spinal cord injury effectively reduced pyroptosis.Furthermore,ceramide synthase 5-induced pyroptosis was dependent on activation of the NLRP3 signaling pathway.Inhibiting ceramide synthase 5 expression in microglia in vivo reduced neuronal apoptosis and promoted recovery of neurological function.Pla2g7 formed a“bridge”between sphingolipid metabolism and ceramide synthase 5-mediated cell death by inhibiting the NLRP3 signaling pathway.Collectively,these findings suggest that inhibiting ceramide synthase 5 expression in microglia after spinal cord injury effectively suppressed microglial pyroptosis mediated by NLRP3,thereby exerting neuroprotective effects.

Fasudil通过TLR4通路抑制脂多糖诱导的小鼠BV-2小胶质细胞TNF-α和IL-1β的表达

目的探讨Fasudil对脂多糖(LPS)诱导BV-2小胶质细胞系促炎细胞因子表达中的作用。方法体外培养BV-2小胶质细胞系,实验分为PBS对照组、LPS刺激组、LPS联合Fasudil干预组,ELISA检测细胞TNF-α、IL-1β的释放,Griess法检测NO释放水平,流式细胞术检测Toll样受体4(TLR4)、TLR2蛋白表达。结果 LPS刺激BV-2细胞可导致TNF-α、IL-1β和NO的释放明显增加,还可导致炎性信号通路中的受体TLR4表达明显增加。Fasudil能明显抑制炎性因子的释放和TLR4的表达。结论 Fasudil可抑制LPS诱导的小胶质细胞NO、TNF-α和IL-1β释放,其作用机制可能与Fasudil下调TLR4通路有关。

乙酰葛根素对Aβ_(25-35)诱导的BV-2小胶质细胞NF-κBp65和iNOS表达的影响

目的:研究乙酰葛根素对β-淀粉样蛋白诱导的小鼠BV-2小胶质细胞核转录因子-κBp65和诱导型一氧化氮合酶表达的影响。方法:体外培养小鼠BV-2小胶质细胞,用凝聚态β-淀粉样蛋白(amyloid-β25-35,Aβ_(25-35))诱导小胶质细胞活化建立阿尔茨海默病炎症细胞模型。实验细胞随机分为6组:空白对照组,Aβ_(25-35)组,Aβ_(25-35)+乙酰葛根素(浓度分别为:0.1,0.4,1.6μmol/L)剂量组和含半胱氨酸的天冬氨酸蛋白水解酶-3(caspase-3)抑制剂(Z-DEVD-fmk)组。在倒置相差显微镜下观察细胞形态的变化;硝酸还原酶法检测乙酰葛根素对一氧化氮(nitric oxide,NO)的影响;利用Western Blot分析乙酰葛根素对NF-κBp65和i NOS蛋白表达的影响;通过Realtime PCR分析乙酰葛根素对NF-κBp65和i NOS基因表达的影响。结果:Aβ_(25-35)诱导后小胶质细胞由静息状态转变为阿米巴样,乙酰葛根素可减轻细胞发生的形态改变。乙酰葛根素呈剂量依赖性的抑制炎性因子NO的产生,抑制NF-κBp65和i NOS的表达。结论:乙酰葛根素可以改善BV-2小胶质细胞的形态变化,减轻BV-2小胶质细胞的炎性反应,其机制可能与其抑制NF-κB信号通路的激活有关,且具有剂量依赖性。

β淀粉样蛋白1-42对BV-2细胞产生一氧化氮功能的刺激作用

目的应用β淀粉样蛋白1-42(β-Amyloid,Aβ1-42)作用于小胶质细胞(microglia,MG),对MG产生一氧化氮(nitric oxide,NO)的作用进行研究。方法应用高度纯化的BV-2小胶质细胞作为体外小胶质细胞模型,测定加入Aβ1-42后细胞上清NO含量及细胞i NOS酶活力;Western blot法测定Aβ对BV-2细胞i NOS蛋白表达的影响,免疫细胞化学方法对i NOS蛋白的表达情况进行观察。结果Aβ1-42可以刺激BV-2细胞产生NO、提高细胞i NOS酶活性、增加i NOS蛋白质表达,以上作用均具有时间及浓度依赖性。结论Aβ1-42在体外可通过提高细胞i NOS酶活性、增加i NOS蛋白质表达而增加NO的分泌,为NO发挥神经元毒性作用创造了条件。

美满霉素对脂多糖诱导的BV-2小胶质细胞肿瘤坏死因子-α表达的影响

目的探讨美满霉素(MC)对脂多糖(LPS)诱导的BV-2小胶质细胞肿瘤坏死因子-α(TNF-α)表达的影响。方法采用相应浓度的MC或LPS(100 ng/ml)对MC组及0.1、1、10、100μmol/L MC+LPS组、LPS组、空白对照组BV-2小胶质细胞进行预处理。ELISA法检测BV-2小胶质细胞TNF-α蛋白的表达,逆转录-PCR检测细胞TNF-αmRNA表达。结果与空白对照组比较,0.1、1μmol/L MC+LPS组及LPS组的TNF-α水平显著升高(均P<0.01)。10、100μmol/L MC+LPS组TNF-α水平显著低于LPS组(均P<0.01)。与空白对照组比较,LPS组及10μmol/L MC+LPS组TNF-αmRNA的表达水平显著增高(均P<0.01)。10μmol/L MC+LPS组TNF-αmRNA表达水平显著低于LPS组(P<0.01)。结论 MC预处理(≥10μmol/L)可显著抑制LPS诱导的小胶质细胞TNF-α的表达。

TLR4介导的BV-2细胞抗HCV固有免疫应答机制初步研究

目的:观察BV-2细胞感染HCV后IFN-β、IL-6分泌和TLR4表达相关性,初步探讨TLR4是否介导参与中枢神经系统抗HCV固有免疫应答及其可能机制。方法:将BV-2细胞接种于24孔培养板,贴壁后换用含20%HCV阳性血清的培养液感染细胞,为HCV实验组,同时设正常血清组和空白对照组。应用流式细胞术检测各组BV-2细胞TLR4蛋白水平的表达;用RT-PCR观察阻断TLR4后各组BV-2细胞TLR4mRNA表达变化;用ELISA检测阻断TLR4后各组BV-2细胞IFN-β、IL-6分泌变化。结果:HCV实验组TLR4表达和IFN-β、IL-6分泌均高于正常血清组及空白对照组(P<0.01);阻断TLR4的HCV实验组TLR4mRNA表达及IFN-β、IL-6分泌明显低于非阻断组(P<0.01)。结论:HCV感染中枢神经系统后,TLR4可通过启动下游细胞因子IL-6、IFN-β等的转录和翻译,介导参与宿主抗HCV固有免疫应答过程。

微小RNA-155对小胶质BV-2细胞炎症因子分泌及吲哚胺2,3-双加氧酶表达的影响

目的:探讨微小RNA-155(miR-155)对小胶质BV-2细胞炎症因子分泌及吲哚胺2,3-双加氧酶(IDO)表达的影响。方法:采用携带miR-155的慢病毒感染小胶质BV-2细胞,以脂多糖(LPS)处理BV-2细胞为对照。观察细胞形态,流式液相芯片检测炎症因子的分泌水平,real-time PCR检测炎症因子和IDO的mRNA表达水平,Western blot法检测细胞因子信号抑制物1(SOCS1)、磷酸化p38 MAPK和IDO蛋白的蛋白水平。结果:携带miR-155的慢病毒成功感染BV-2细胞,其miR-155表达水平高于LPS处理组和阴性病毒感染组(P<0.01)。miR-155促进BV-2细胞白细胞介素6(IL-6)、肿瘤坏死因子α(TNF-α)、单核细胞趋化蛋白1(MCP-1)和IL-10分泌,抑制IL-12分泌,上调IL-6、TNF-α、IL-10和IDO的mRNA表达,同时升高IDO蛋白表达水平和p38 MAPK蛋白磷酸化水平,下调SOCS1蛋白表达(P<0.01)。LPS刺激BV-2细胞分泌炎症因子IL-6、TNF-α、MCP-1和IL-12,上调IL-6、TNF-α和IDO mRNA表达,同时上调IDO、p-p38 MAPK和SOCS1的蛋白水平。结论:miR-155促进小胶质BV-2细胞相关炎症因子分泌和IDO蛋白表达,可能与SOCS1和p38 MAPK信号通路相关。

川芎嗪通过AMPK-NFκB信号通路抑制BV-2小胶质细胞促炎性细胞因子基因表达

目的观察川芎嗪(tetramethylpyrazine,TMP)对Aβ25-35诱导的BV-2小鼠小胶质细胞促炎性细胞因子基因表达及对一磷酸腺苷激活的蛋白激酶(adenosine monophosphate-activated protein kinase,AMPK)-核因子κB(nuclear factor kappa B,NFκB)信号通路的影响。方法采用Aβ25-35激活BV-2细胞的炎性反应,测定TMP高、中、低剂量(终浓度分别为100、30、10μmol/L)对Aβ25-35诱导的BV-2细胞白细胞介素-1β(interleukin-1β,IL-1β)、白细胞介素-6(interleukin-6,IL-6)、肿瘤坏死因子-α(tumor necrosis factorα,TNF-α)及诱导型一氧化氮合酶(inducible nitric oxide synthase,iNOS)mRNA表达水平的影响。在AMPK激活剂(AICAR)及抑制剂(化合物C)存在下,检测TMP对AMPK及p65(NFκB亚基)磷酸化的影响。结果 TMP高、中剂量可明显抑制BV-2细胞中IL-1β、IL-6、TNF-α和iNOS基因mRNA表达水平(P<0.01),高剂量TMP可激活BV-2细胞中AMPK(P<0.01),并抑制p65磷酸化(P<0.01)。结论 TMP通过激活BV-2细胞中AMPK活性,抑制NFκB活化,进而抑制促炎性细胞因子基因的表达。

脂多糖对BV-2细胞的形态及肿瘤坏死因子-α表达的影响

目的探讨脂多糖对BV-2细胞的形态及肿瘤坏死因子-α（TNF-α）表达的影响。方法 DMEM高糖培养基中培养的BV-2细胞平均分为空白对照组与脂多糖处理组。脂多糖处理组BV-2细胞采用含100ng/ml脂多糖的培养基培养24 h;空白对照组用PBS替代脂多糖。采用免疫组化染色法观察BV-2细胞的形态及TNF-α蛋白的表达,采用酶联免疫吸附试验（ELISA）法检测BV-2细胞培养上清液中TNF-α的浓度。结果空白对照组BV-2细胞形态呈上皮细胞样,每个细胞有2~3个突起,突起较细长,细胞核较小。脂多糖处理组BV-2细胞多数聚集成团,大部分胞体肥大、饱满,细胞核大而圆,核仁明显,胞体突起短小,形态均具有小胶质细胞激活后形态特征。BV-2细胞中TNF-α蛋白的阳性表达均主要在胞浆中,为棕黄色颗粒。空白对照组BV-2细胞TNF-α蛋白阳性表达产物的OD值（5.46±0.87）明显低于脂多糖处理组（53.01±5.72）,差异有统计学意义（t=26.01,P〈0.01）。空白对照组BV-2细胞培养上清液中TNF-α浓度为（218.13±24.10）pg/ml,脂多糖处理组BV-2细胞培养上清液中TNF-α浓度为（1098.69±72.18）pg/ml,两组间比较差异有统计学意义（t=23.14,P〈0.01）。结论脂多糖可显著诱导BV-2细胞系TNF-α的表达,同时可显著改变BV-2细胞的形态。

PFOS对BV-2细胞的炎性损伤及机制研究

目的:探讨环境内分泌干扰物全氟辛磺酸(perfluorooctane suifonate,PFOS)对小鼠小胶质瘤细胞BV-2的损伤作用及其炎性反应。方法:利用体外培养的小胶质细胞,给予不同浓度和作用时间的PFOS进行染毒,通过MTT法检测BV-2细胞活力;实时定量PCR的方法观察诱导型一氧化氮合酶(inducible nitric oxide synthesis,i NOS)、白介素(interleukin,IL)-6和肿瘤坏死因子(tumor necrosis factor,TNF)-αm RNA的表达。ELISA法检测炎性因子IL-6,免疫蛋白印迹法检测核转录因子kappa B(nuclear factor-kappa B,NF-κB)等信号蛋白表达情况。结果:不同浓度PFOS对BV-2细胞染毒12、24 h后,细胞活力下降,引起明显的细胞损伤。ELISA结果显示,PFOS作用BV-2 24 h后,细胞炎性因子IL-6分泌增加。此外,PFOS还可引起i NOS、IL-6基因表达上调,而TNF-α表达有下降趋势。PFOS与细胞孵育后,炎性通路NF-κB明显激活,表现为磷酸化程度升高。且随染毒浓度的增加,p-NF-κB的表达有上升趋势;此外,随染毒时间的增加,p-NF-κB的表达亦有上升趋势。结论:PFOS可引起BV-2细胞活力降低,激活NF-κB通路,促进炎性因子的释放,该途径可为阐明PFOS引起的神经系统损伤的分子机制提供理论依据。