Immunoregulatory polysaccharides from Apocynum venetum L.flowers stimulate phagocytosis and cytokine expression via activating the NF-κB/MAPK signaling pathways in RAW264.7 cells

Two immunomodulatory polysaccharides(Vp2a-Ⅱ and Vp3) were isolated and identified from Apocynum venetum L. flowers, and their innate immune-stimulating functions and working mechanisms were evaluated in RAW264.7 cells. Both the level of released nitric oxide(NO) and expression of inducible nitric oxide synthase(iNOS) m RNA were significantly enhanced in the RAW264.7 macrophages cells treated by Vp2a-Ⅱ and Vp3. Vp2a-Ⅱ(100–800 μg/m L) and Vp3(400 μg/mL) could significantly increase the phagocytic activity of RAW264.7 cells and the secretion and m RNA expression of TNF-α and IL-6 in a concentrationdependent manner through affecting mitogen-activated protein kinase(MAPK) activity and nuclear factor κB(NF-κB) nuclear translocation. Vp2a-Ⅱ might activate the MAPK signaling pathways and induce the nuclear translocation of NF-κB p65, whilst Vp3 likely activated the NF-κB and MAPK signaling pathways without influencing the p38 MAPK route.

Role of Endoplasmic Reticulum Stress in Silica-induced Apoptosis in RAW264.7 Cells＊

Objective We investigated the role of endoplasmic reticulum stress(ERS) in silica-induced apoptosis in alveolar macrophages in vitro. Methods RAW264.7 cells were incubated with 200 μg/mL silica for different time periods. Cell viability was assayed by the MTT assay. Cell apoptosis was evaluated by DAPI staining, flow cytometry analysis, and Western blot analysis of caspase-3. Morphological changes in the endoplasmic reticulum were observed by transmission electron microscopy. The expression of ERS markers binding protein(BiP) and CCAAT-enhancer-binding protein homologous protein(CHOP) was examined by Western blotting and real-time PCR. As an inhibitor of ERS, 4-phenylbutyric acid(4-PBA) was used in the experiments. Results Silica exposure induced nuclear condensation and caspase-3 expression in RAW264.7 cells. The number of apoptotic cells increased after silica exposure in a time-dependent manner. Silica treatment induced expansion of the endoplasmic reticulum. In addition, the expression of BiP and CHOP increased in silica-stimulated cells. Furthermore, 4-PBA treatment inhibited silica-induced endoplasmic reticulum expansion and the expression of Bi P and CHOP. Moreover, 4-PBA treatment attenuated nuclear condensation, reduced apoptotic cells, and downregulated caspase-3 expression in silica-stimulated cells. Conclusion Silica-induced ERS is involved in the apoptosis of alveolar macrophages.

Zhikang Capsule Ameliorates Inflammation, Drives Polarization to M2 Macrophages, and Inhibits Apoptosis in Lipopolysaccharide-induced RAW264.7 Cells

Objective:To explore the anti-inflammatory effect of the traditional Chinese medicine Zhikang capsule(ZKC)on lipopolysaccharide(LPS)-induced RAW264.7 cells.Methods:Safe concentrations of ZKC(0.175,0.35,and 0.7 mg/mL)were used after the half-maximal inhibitory concentration(IC_(50))of RAW264.7 cells was calculated through the CCK-8 assay.In addition,the optimal intervention duration of ZKC(0.7 mg/mL)on RAW264.7 cells was determined to be 6 h,since all proinflammatory mediators[tumor necrosis factor-alpha(TNF-α),interleukin-1 beta(IL-1β),inteleukin-6(IL-6),cyclooxygenase-2(COX-2),inducible nitric oxide synthase(iNOS),and monocyte chemotactic protein-1(MCP-1)]had a decreasing tendency and relatively down-regulated mRNA expression levels as compared with other durations(4,8,and 12 h).RAW264.7 cells were pretreated with ZKC at various concentrations(0.175,0.35 and 0.7 mg/mL)for 6 h and then stimulated with LPS(1 μg/mL)for an additional 12 h.Results:In terms of inflammation,ZKC could reverse LPS-induced upregulation of TNF-α,IL-1β,IL-6,COX-2,iNOS,and MCP-1 at both the mRNA and protein levels in RAW264.7 cells in a dose-dependent manner.In terms of the NF-κB signaling pathway,ZKC could reduce phosphorylated p65 and promote M2 polarization of RAW264.7 cells under LPS stimulation in a dose-dependent manner.Moreover,ZKC exhibited a protective effect on macrophages from apoptosis.Conclusion:ZKC exhibited obvious anti­inflammatory and anti-apoptotic effects on LPS-induced RAW264.7 cells at the cellular level,and a weakened NF-κB signaling pathway may be a potential significant target.

Ketamine Promotes Inflammation through Increasing TLR4 Expression in RAW264.7 Cells

Summery: Ketamine(KTM), a N-methyl-D-aspartate(NMDA) receptor antagonist, was found to has an anti-inflammatory effect, but some patients suffered from exacerbated pro-inflammatory reactions after anesthesia with KTM. The present study was aimed to examine the underlying mechanism of pro-inflammatory effects of KTM. In this study, RAW264.7 cells were exposed to KTM and NMDA alone or combined for 30 min before lipopolysaccharide(LPS) stimulation. The expression levels of IL-6 and TNF-α were detected by RT-PCR and ELISA, and those of NMDA receptors by RT-PCR in RAW264.7 cells. Additionally, the TLR4 expression was determined by RT-PCR and flow cytometry, respectively. The results showed that in RAW264.7 cells, KTM alone promoted the TLR4 expression, but did not increase the expression of IL-6 or TNF-α. In the presence of LPS, KTM caused a significantly higher expression of IL-6 and TNF-α than LPS alone. NMDA could neither alter the IL-6 and TNF-α m RNA expression, nor reverse the enhanced expression of IL-6 and TNF-α m RNA by KTM in LPS-challenged cells. After TLR4-si RNA transfection, RAW264.7 cells pretreated with KTM no longer promoted the IL-6 and TNF-α expression in the presence of LPS. In conclusion, KTM accelerated LPS-induced inflammation in RAW264.7 cells by promoting TLR4 expression, independent of NMDA receptor.

The compounds fromDerris laxiflora Benth suppresses lipopolysaccharideinduced inflammatory response in murine Raw264.7 cells

OBJECTIVE The emerging role of chronic inflammation is the major degenerative diseases of modern society such as periodontitis,atherosclerosis,rheumatoid arthritis,Parkinson′s disease and even cancer.Eight components were isolated from Derris laxiflora Benth.,In this study,we found these compounds from Derris laxiflora Benth suppress lipopolysaccharide-induced inflammatory response in murine macrophage(RAW 264.7)cells.METHODS RAW 264.7cells were cultured in DMEM media supplemented with 10%(V/V)heated-inactivated FBS,penicillin 100U·mL-1 and streptomycin 100μg·mL-1.The cells were incubated at 37℃in a humidified atmosphere of 5%CO2in air.RAW264.7cells were seeded in a 24-well plate at a density of 2×105 mL-1 and then incubated with or without LPS(100ng·mL-1)in the absence or presence of compounds for 24 h.Effects of these isolates on NO production were measured indirectly by analysis of nitrite levels using the Griess reaction.Quercetin was used as a positive control.RESULTS ight components were isolated from Derris laxiflora Benth.,including three new pterocarpans 7,6′-dihydroxy-3′-methoxypterocarpan(1),derrispisatin(2),derriscoumaronochromone(3)and three new flavonoids cis-3,4′-dihydroxy-5,7-dimethoxyflavan(4),derriflavanone B(5),iso-lupinenol(6)as well as two known ones,lonchocarpol A(7)and lonchocarpol D(8).The structures of these new compounds were determined by analysis of their spectroscopic data.Raw264.7 cells were treated with the compounds from Derris laxiflora Benth for 24 h.Among them,compounds 5,7 and 8 significantly suppressed the NO production in LPS-treated RAW264.7 cells with IC50 values<10μg·mL-1.CONCLUSION In this study,we found that compounds from Derris laxiflora Benth suppresses lipopolysaccharide-induced inflammatory response in murine Raw264.7 cells.

Raw264.7 Cells Secrete Fibroblast Growth Stimulating Activity after Differentiation to Macrophages by Stimulation with Lipopolysaccharide

Raw264.7 cells are monocytic cells that can differentiate to activated macrophages after lipopoly-saccharide (LPS) stimulation. Here, we analyzed the factors secreted by Raw264.7 cells in response to LPS. The culture media of LPS-treated Raw264.7 cells was able to stimulate growth in MEF1F2 and NIH3T3 mouse fibroblast cell lines. We identified five secreted and LPS-induced chemokines, CCL2, CCL5, CCL12, CxCL2, and CxCL10, by microarray analysis and tested their stimulatory activity. We used commercially available bacterially expressed proteins, and found only CCL12, CxCL2 and CxCL10 stimulated growth in MEF1F2 and NIH3T3 cells. The saturation density of the cells was also increased. They were not able to stimulate growth in v-Src transformed MEF1F2 or SWAP-70 transformed NIH3T3 cells. We examined signaling pathways activated by these three factors. We found that ERK and p38 MAP kinase were activated and were required for the activity to stimulate the cell growth. Other pathways including phosophatidylinositol-3 kinase (PI3K), NFκB pathways were not activated. These results suggest that Raw264.7 cells secretes growth stimulation factors for fibroblasts when differentiated to macrophages implicating that fast growth of them is related to inflamation although the reason is still unclear.

Demethylbelamcandaquinone B from Marantodes pumilum var.alata(Blume)Kuntze inhibits osteoclast differentiation in RAW264.7 cells

Objective:To investigate the bone-resorbing effect of demethylbelamcandaquinone B(Dmcq B)extracted from Marantodes pumilum var.alata on osteoclast differentiation in RAW264.7 cells.Methods:RAW264.7 macrophages were differentiated using RANKL into osteoclast-like cells.Then,they were treated with 10μg/mL Marantodes pumilum var.alata crude aqueous extract,5μg/mL dichloromethane fraction,and 0.6μg/mL Dmcq B and 0.06μg/mL estradiol.Tartrate-resistant acid phosphatase 5b(TRACP 5b)as an osteoclast phenotypic marker was determined by TRACP staining and TRACP 5b colometric assay,and bone-resorbing pits were examined.The gene expression of pro-inflammatory cytokines(TNF-αand IL-6)was measured.Moreover,the protein expressions of pro-inflammatory cytokines(TNF-αand IL-6)and estrogen receptors were evaluated.Results:Marantodes pumilum var.alata crude aqueous extract and Dmcq B inhibited RANKL-stimulated osteoclast differentiation as evidenced by size reduction of giant multinucleated osteoclast cells,decreased TRACP 5b activity as well as the subsiding of resorbed pit area compared with normal control.In addition,they reduced the gene and protein expressions of TNF-αand IL-6.Marantodes pumilum var.alata,Dmcq B,and estradiol treatments increased the protein expressions of estrogen receptors alpha and beta in osteoclasts.Conclusions:Marantodes pumilum var.alata and its active compound,Dmcq B can inhibit osteoclast differentiation.

Hyperbaric Oxygen Stimulates the Proliferation and Differentiation of Raw264.7 Cells

Background: Hyperbaric Oxygen (HBO) Therapy improves the outcome of various types of sugery, such as postoperative bone grafts, fixation of jaw fractures, and osteoplasty of jaw deformities. Therefore, it is important to determine the effects of HBO on bone regeneration. The purpose of this study was to clarify the influence of a hyperbaric oxygen environment on bone regeneration at the osteoclastogenic cytokines level. Sample & Methods: RAW264.7 cells were stimulated under the various conditions by using a hyperbaric oxygen chamber. We evaluated the ability of the RAW264.7 macrophages to proliferate, differentiate and produce various osteoclastogenic cyto-kines. Results: A hyperbaric oxygen (HBO) environment and high concentration oxygen (HCO) environment increase cellular proliferation in a time-dependent manner. On the other hand, a HCO environment and a hyperbaric with room air (HBA) environment enhanced the differentiation of RAW264.7 cells. In addition, NFATc1 and c-Fos were increased by both the HBA environment and HCO environment. However, the effects of HBA and HCO environments were in contrast with each other with regard to RANK, TNF-α, C-FMS and TRAP. Conclusions: It was suggested that a HBO environment influenced the bone regeneration by altering osteoclastogenic cytokines level, and that a HCO environment and HBA environment acted independently on the proliferation and differentiation of macrophages and the secretion of osteoclastogenic cytokines, and that they acted in concert in a hyperbaric oxygen environment to induce conditions favoring regeneration.

Anti-oxidant and Anti-inflammatory Effects of Ethanol Extract from Polygala sibirica L.var megalopha Fr.on Lipopolysaccharide-Stimulated RAW264.7 Cells

Objective To investigate the anti-oxidant and anti-inflammatory effects of ethanol extract of Polygala sibirica L.var megalopha Fr.(EEP)on RAW264.7 mouse macrophages.Methods RAW264.7 cells were pretreated with 0–200µg/mL EEP or vehicle for 2 h prior to exposure to 1µg/mL lipopolysaccharide(LPS)for 24 h.Nitric oxide(NO)and prostaglandin(PGE2)production were determined by Griess reagent and enzyme-linked immunosorbent assay(ELISA),respectively.The mRNA levels of inducible nitric oxide synthase(iNOS),cyclooxygenase-2(COX-2),tumor necrosis factorα(TNF-α),interleukin-1beta(IL-1β),and IL-6 were determined using reverse transcription polymerase chain reaction(RT-PCR).Western blot assay was used to determine the protein expressions of iNOS,COX-2,phosphorylation of extracellular regulated protein kinases(ERK1/2),c-Jun N-terminal kinase(JNK),inhibitory subunit of nuclear factor Kappa B alpha(IκB-α)and p38.Immunofluorescence was used to observe the nuclear expression of nuclear factor-κB p65(NF-κB p65).Additionally,the anti-oxidant potential of EEP was evaluated by reactive oxygen species(ROS)production and the activities of catalase(CAT)and superoxide dismutase(SOD).The 2,2-diphenyl-1-picrylhydrazyl(DPPH),hydroxyl(OH),superoxide anion(O2−)radical and nitrite scavenging activity were also measured.Results The total polyphenol and flavonoid contents of EEP were 23.50±2.16 mg gallic acid equivalent/100 g and 43.78±3.81 mg rutin equivalent/100 g.With EEP treatment(100 and 150µg/mL),there was a notable decrease in NO and PGE2 production induced by LPS in RAW264.7 cells by downregulation of iNOS and COX-2 mRNA and protein expressions(P<0.01 or P<0.05).Furthermore,with EEP treatment(150µg/mL),there was a decrease in the mRNA expression levels of TNF-α,IL-1βand IL-6,as well as in the phosphorylation of ERK,JNK and p38 mitogen-activated protein kinase(MAPK,P<0.01 or P<0.05),by blocking the nuclear translocation of NF-κB p65 in LPS-stimulated cells.In addition,EEP(100 and 150µg/mL)led to an increase in the anti-oxidant enzymes activity of SOD and CAT,with a concomitant decrease in ROS production(P<0.01 or P<0.05).EEP also indicated the DPPH,OH,O2−radical and nitrite scavenging activity.Conclusion EEP inhibited inflammatory responses in activated macrophages through blocking MAPK/NF-κB pathway and protected against oxidative stress.

次苷酸查尔酮对LPS诱导的RAW264.7细胞iNOS和COX-2表达的影响

补骨脂为豆科植物补骨脂(Psoraleacorylifolia L.)果实,具有温肾助阳、温脾止泻的功效[1],临床上被用于治疗皮肤病、肾炎、骨折等[2-3]。次苷酸查尔酮(corylifol A,CYA)是中药补骨脂的活性成分之一,是一种异黄酮类化合物,具有抗炎、抗菌、抗氧化、抗骨质疏松的特性[4-5]。有研究表明,CYA能明显抑制破骨细胞的分化,且能明显降低LPS诱导的巨噬细胞一氧化氮(NO)的生成[6-7]。

匹莫齐特对脂多糖诱导RAW264.7细胞诱导型一氧化氮合成酶表达的调控及其作用机制

目的运用脂多糖(LPS)诱导小鼠巨噬细胞RAW264.7细胞株,探究匹莫齐特(Pimozide)对一氧化氮和诱导型一氧化氮合成酶(iNOS)合成的影响和作用机制。方法用含10%胎牛血清、100 U·mL^(-1)的青链霉素DMEM培养液将RAW264.7细胞稀释为每孔2×105个接种于24孔板中进行培养,分为空白对照组(仅含DMEM培养液+RAW264.7细胞)、Pimozide组(仅含RAW264.7细胞和10μmol·L^(-1)Pimozide培养液)、LPS诱导(LPS 1 mg·L^(-1))组(LPS+RAW264.7细胞)、药物处理组[含细胞和不同浓度药物,包括Pimozide低(LPS+2.5μmol·L^(-1))、中(LPS+5μmol·L^(-1))、高(LPS+10μmol·L^(-1))组]。各组培养上清液中一氧化氮水平测定采用Griess法进行检测。采用实时定量聚合酶链反应(RT-PCR)法和免疫蛋白印迹法分别检测iNOS mRNA表达水平和iNOS和磷酸化的信号传导及转录激活因子通路-5的蛋白表达相对水平。结果用含10%胎牛血清、100 U·mL^(-1)的青链霉素DMEM培养液培养RAW264.7细胞24 h后,各组培养上清液一氧化氮表达水平差异有统计学意义(F=25.69,P<0.05);Pimozide低(LPS+2.5μmol·L^(-1))、中(LPS+5μmol·L^(-1))、高(LPS+10μmol·L^(-1))组一氧化氮释放的抑制率差异有统计学意义(F=132.49,P<0.05)。各组iNOS mRNA和蛋白水平表达差异有统计学意义(F=118.59和23.37,P<0.05),同时发现各组磷酸化的信号传导及转录激活因子通路-5/信号传导及转录激活因子通路-5比值差异有统计学意义(F=12.07,P<0.05)。结论Pimozide可抑制RAW264.7细胞中iNOS表达和一氧化氮的生成,其作用机制可能与抑制磷酸化的信号传导及转录激活因子通路-5的生成相关。

人参皂苷F2对LPS诱导RAW264.7细胞炎症反应的改善作用

作为人参的主要生物活性物质,多数人参皂苷已被证实具有良好的抗炎作用,但是其抗炎机制研究较少,尤其是人参皂苷F2。因此,该研究基于脂多糖(Lipopolysaccharide,LPS)刺激RAW264.7细胞产生炎症,构建体外细胞炎症模型,探究人参皂苷F2的抗炎作用。细胞活力实验表明人参皂苷F2在100μmol/L内对细胞无毒性作用,为安全浓度范围。人参皂苷F2可以显著抑制LPS刺激RAW264.7细胞NO释放,且呈剂量依赖性抑制(0~100μmol/L)。人参皂苷F2(50、100μmol/L)也呈剂量依赖性抑制一氧化氮合酶(iNOS)和肿瘤坏死因子(TNF-α)的mRNA表达,100μmol/L时显著抑制iNOS和TNF-α的mRNA表达。经人参皂苷F2处理可显著下调iNOS蛋白表达,但对COX2蛋白表达无显著促进作用(P>0.05)。此外,经扫描电镜(SEM)观察,100μmol/L人参皂苷F2处理可以显著改善LPS刺激RAW264.7细胞的细胞形态改变。蛋白印迹表明,人参皂苷F2提高了PDK1、AKT、IκB-α蛋白的表达,降低了AKT蛋白磷酸化、NF-κB的核易位。该文研究结果表明人参皂苷F2具有较好的抗炎作用,并可能通过AKT/IκB-α/NF-κB信号通路发挥其抗炎作用,可为相关天然抗炎药物的开发提供理论支撑。

桉柠蒎油抑制脂多糖诱导的RAW264.7细胞炎症因子产生的作用及其机制研究

目的探究桉柠蒎油(ELP)抑制脂多糖(LPS)刺激的RAW264.7细胞炎症因子产生的作用及作用机制。方法构建LPS刺激的RAW264.7炎症细胞模型。采用噻唑蓝(MTT)法检测细胞活性;采用Griess法检测一氧化氮(NO)的产生;采用酶联免疫吸附法(ELISA)测定LPS处理后培养液中炎症因子的浓度;采用Western-blot法检测蛋白表达水平;采用免疫荧光技术检测LPS处理后核转录因子κB亚基(p65)、激活子蛋白1亚基(c-Jun)和干扰素调节因子3(IRF3)的入核情况。结果ELP在6.25~400μg/mL的剂量范围内对LPS处理的RAW264.7细胞活力没有明显抑制作用。ELP(50~300μg/mL)能有效地抑制LPS诱导的RAW264.7细胞NO、前列腺素E2(PGE2)、肿瘤坏死因子-α(TNF-α)、白介素-6(IL-6)、巨噬细胞炎性蛋白1α(MIP-1α)、单核细胞趋化蛋白1(MCP-1)、白介素-1β(IL-1β)和受激活调节正常T细胞表达和分泌因子(Rantes)的产生。ELP能剂量依赖性地降低Toll样受体4(TLR4)信号通路关键蛋白kappa B抑制因子激酶α/β(IKKα/β)、TANK结合激酶1(TBK1)、干扰素调节因子3(IRF3)、细胞外调节蛋白激酶(ERK1/2)、p38、p65、核因子kappa B抑制蛋白α(IκBα)、c-Jun和c-Jun氨基末端激酶(JNK)的磷酸化水平。ELP同时能抑制LPS诱导的RAW264.7细胞p65、c-Jun和IRF3的入核。结论ELP能剂量依赖性地抑制LPS诱导的RAW264.7细胞炎症因子的产生,其作用机制与阻断TLR4/NF-κB、TLR4/AP-1和TLR4/IRF3信号通路有关。

模拟失重对小鼠巨噬细胞RAW264.7生物学功能的影响

目的通过2D回转器回转细胞模拟失重生物学效应,探讨模拟失重对小鼠巨噬细胞(RAW264.7)多种生物学功能的影响特点,为深化空间失重免疫抑制机制研究提供理论依据和数据支撑。方法将RAW264.7细胞分为对照组(NG组)、模拟失重组(SMG组),利用2D回转器模拟失重72 h后,采用CCK-8法和EdU法检测小鼠RAW264.7巨噬细胞的增殖能力变化;细胞划痕实验和Transwell小室法检测巨噬细胞迁移功能的变化;探针DCFH-DA标记,倒置荧光显微镜观察和拍照检测巨噬细胞分泌活性氧(ROS)的变化。结果RAW264.7巨噬细胞模拟失重72 h后增殖受到抑制,CCK-8实验结果显示,NG组的细胞增殖速率显著高于SMG组(P<0.05);EdU染色结果显示,SMG组EdU掺入RAW264.7细胞核的量较NG组减少(P<0.01)。细胞划痕、Transwell实验检测表明72 h模拟失重对巨噬细胞的迁移能力有明显影响,与NG组相比,模拟失重后RAW264.7细胞迁移能力增强(P<0.05);探针DCFH-DA标记检测提示模拟失重对巨噬细胞分泌ROS有明显抑制作用(P<0.01)。结论回转模拟失重对RAW264.7细胞的生物学功能具有影响,表现为RAW264.7迁移运动能力增强,细胞增殖与ROS分泌能力受到抑制。

绿原酸抑制LPS诱导的RAW264.7细胞炎症及机制探索

目的明确绿原酸对脂多糖(lipopolysaccharide,LPS)诱导的巨噬细胞RAW264.7炎症的抗炎作用,揭示其可能的分子机制。方法以CCK-8法检测不同浓度绿原酸干预后RAW264.7的细胞活性;采用LPS刺激巨噬细胞RAW264.7,预制细胞炎性状态,设置空白对照组(K组,n=3)、模型对照组(L组,n=3)和实验组(S组,n=3)分别给药,动态观察细胞形态;分别于24h及48h获取细胞沉淀及上清,以酶联免疫吸附(enzyme-linked immunosorbent assay,ELISA)法检测细胞上清中炎性细胞因子白细胞介素-1β(interleukin-1beta,IL-1β)、单核细胞趋化蛋白-1(monocyte chemoattractant protein-1,MCP-1)及精氨酸酶-1(arginase-1,Arg-1)的浓度;采用实时荧光定量PCR(quantitative real-time polymerase chain reaction,RT-qPCR)法检测前列腺素内过氧化物合酶2(prostaglandin-endoperoxide synthase 2,PTGS2)、转化生长因子β1(transforming growth factor-beta1,TGF-β1)、高迁移率族蛋白1(high mobility group box-1,HMGB1)及核转录因子-κB(nuclear transcription factor-kappaB,NF-κB)的mRNA表达。结果1μg/ml的LPS成功预制RAW264.7细胞炎性状态;12.5~200.0μg/ml的绿原酸对RAW264.7无明显毒性,50μg/ml及200μg/ml的绿原酸对RAW264.7细胞有明显的增殖作用(P<0.05);与模型对照组比较,实验组上清中IL-1β蛋白含量明显降低,Arg-1的含量明显升高(P<0.05);与模型对照组比较,50μg/ml的绿原酸显著降低LPS诱导的炎性细胞中NF-κB、TGF-β1、PTGS2及HMGB1的mRNA表达(P<0.05)。结论绿原酸对LPS诱导的RAW264.7炎性反应有明确抑制作用,可能与调控HMGB1介导的NF-κB相关通路分子表达有关。

鞣花酸通过TLR4-SRC/MAPK/NF-κB途径抑制脂多糖诱导RAW264.7巨噬细胞的炎症反应

目的基于Toll样受体4(TLR4)-酪氨酸激酶(SRC)/丝裂原活化蛋白激酶(MAPK)/核转录因子-κB(NF-κB)通路探讨鞣花酸的抗炎机制。方法采用不同浓度(0、0.5、5、25、50、75、100μmol·L^(-1))鞣花酸对RAW264.7巨噬细胞[或脂多糖(LPS)诱导的RAW264.7细胞]干预24 h,噻唑蓝(MTT)法检测RAW264.7巨噬细胞存活率,筛选最适给药浓度。实验分为空白对照组,模型组(0.5 mg·L^(-1)LPS),阳性对照地塞米松组(10μmol·L^(-1)),鞣花酸(5、25、50μmol·L^(-1))给药组。Griess法检测细胞上清液中一氧化氮(NO)的含量;采用ELISA法检测细胞上清液中前列腺素-2(PGE2)、白细胞介素-6(IL-6)、白细胞介素-1β(IL-1β)和肿瘤坏死因子-α(TNF-α)的表达水平;采用Western blot法检测诱导型一氧化氮合酶(iNOS)、环氧合酶-2(COX-2)蛋白以及TLR4-SRC/MAPK/NF-κB通路相关蛋白的表达水平。结果MTT结果筛选出鞣花酸的干预浓度为5~50μmol·L^(-1)。与空白对照组比较,模型组PGE_(2)、NO和炎症因子IL-6、IL-1β、TNF-α表达显著升高(P<0.01);炎症标志物iNOS、COX-2蛋白表达水平显著升高(P<0.01),说明炎症模型建立成功。与模型组比较,鞣花酸能显著抑制LPS诱导NO、PGE_(2)的产生和降低TNF-α、IL-1β、IL-6水平(P<0.05,P<0.01),降低i NOS、COX-2蛋白表达水平(P<0.05,P<0.01),且呈浓度依赖性;显著抑制TLR4蛋白的表达水平以及SRC、P38、JNK、p65、IκBα蛋白的磷酸化水平,并呈浓度依赖性。但对ERK1/2蛋白磷酸化没有显示出明显的抑制作用。结论鞣花酸可能通过TLR4-SRC/MAPK/NF-κB信号通路的调控抑制LPS诱导RAW264.7巨噬细胞的炎症反应,具体的调控机制有待进一步研究。

文冠果叶黄酮对巨噬细胞RAW264.7细胞因子及TLR2受体的影响

通过四甲基偶氮噻唑蓝(MTT)比色法分析文冠果叶黄酮(XLF)对巨噬细胞RAW 264.7增殖活力的影响,酶联免疫吸附测定法检测巨噬细胞RAW 264.7分泌的细胞因子含量;通过XLF处理Toll样受体2(TLR2)抗体作用的巨噬细胞,研究TLR2受体对该细胞因子的介导作用。结果表明:当XLF质量浓度为320μg/mL时,巨噬细胞RAW 264.7分泌的NO、白细胞介素-2(IL-2)、肿瘤坏死因子-α(TNF-α)和肿瘤坏死因子-β(TNF-β)细胞因子最多,且与空白对照差异极显著,但都小于脂多糖(LPS);且与未加入TLR2抗体相比,加入了TLR2抗体的巨噬细胞减少了各细胞因子的分泌,且差异均极显著。XLF可促进巨噬细胞RAW 264.7的增殖及细胞因子的分泌,并且可能通过TLR2受体介导。

葛根素通过Notch1信号通路抑制Raw264.7细胞向破骨细胞的分化

背景:前期研究表明葛根素干预后破骨细胞的分化被抑制,Notch1、HES1、Jagged1等Notch信号通路相关蛋白表达量下降,但Notch1信号通路对于葛根素抑制破骨细胞分化的作用机制尚不明确。目的:探究Notch信号通路对葛根素抑制小鼠巨噬细胞Raw264.7分化为破骨细胞的影响。方法:将Raw264.7细胞分为7组干预培养,空白对照组采用DMEM高糖完全培养基培养,破骨细胞诱导组采用破骨诱导培养基培养,葛根素干预组在破骨诱导的同时加入50μmol/L葛根素培养,葛根素+Notch1 si RNA对照组、葛根素+Notch1 si RNA组、葛根素+Notch1过表达对照组、葛根素+Notch1过表达组分别采用Notch1 si RNA对照序列、Notch1 si RNA序列、Notch1过表达对照质粒、Notch1过表达质粒转染Raw264.7细胞后,加入破骨诱导培养基和葛根素进行培养。培养7 d后,采用抗酒石酸酸性磷酸酶染色观察破骨细胞的数量和大小,F-actin染色观察破骨细胞骨架形成情况,RT-PCR检测破骨细胞形成标志物的基因表达水平。结果与结论:(1)抗酒石酸酸性磷酸酶染色显示:葛根素干预可以抑制破骨细胞的生成,Notch1沉默会进一步减少破骨细胞的生成数量,Notch1过表达后破骨细胞生成数量明显增加;(2)F-actin染色显示:Raw264.7细胞经破骨诱导可以形成边界清晰的F-actin环,葛根素干预会抑制细胞骨架的形成,Notch1沉默会增强葛根素的抑制作用,而Notch1过表达则能减弱葛根素的抑制作用;(3)RT-PCR检测显示,葛根素可以抑制抗酒石酸酸性磷酸酶、组织蛋白酶K和c-Fos的m RNA表达,Notch1沉默后上述3个因子的m RNA表达进一步降低,Notch1过表达后上述3个因子的m RNA表达增加。结果表明:Notch信号通路在Raw264.7细胞分化为破骨细胞的过程中发挥作用,葛根素通过抑制Notch信号通路抑制Raw264.7细胞分化为破骨细胞。

四黄清灵液通过MAPKs/NF-κB信号通路保护脂多糖诱导的RAW264.7细胞炎症反应

目的 研究中药复方四黄清灵液水提物对脂多糖(LPS)诱导小鼠巨噬细胞RAW264.7炎症的保护作用及其作用机制。方法 把处于对数生长期的RAW264.7细胞随机分为Control、LPS组、SHQLY浓度组,采用CCK-8试剂检测SHQLY提取物对RAW264.7细胞的活性影响,酶联免疫法检测培养基上清中TNF-α和IL-6的含量,后续选取10μg和20μg两个浓度,利用DCFH-DA荧光探针法测定活性氧,Western-blot法检测P-ERK/ERK、P-p38/p38、P-JNK/JNK、P-Iκβα/Iκβα和P-NF-κB/NF-κB等蛋白表达情况,激光共聚焦显微镜观察经免疫荧光染色NF-κB入核情况。结果 SHQLY可以呈剂量依赖的抑制LPS诱导RAW264.7细胞炎症反应,可以抑制IL-6和TNF-α炎症因子的释放,抑制ROS的产生,Western-blot结果显示SHQLY通过抑制丝裂原活化蛋白激酶(MAPKs)和核因子(NF-κB)信号通路中磷酸化蛋白P-ERK、P-p38、P-JNK、P-IKβ-α和P-p65等蛋白磷酸化,同时抑制NF-κB转移入核。结论 SHQLY抑制LPS诱导的RAW264.7细胞炎症,可能的抗炎机制是其抑制MAPKs/NF-κB信号通路蛋白磷酸化相关。

防风中5-O-甲基维斯阿米醇苷对脂多糖诱导RAW264.7细胞炎症模型的抗炎作用研究

目的 研究中药防风中5-O-甲基维斯阿米醇苷对脂多糖(LPS)诱导的小鼠RAW264.7细胞炎症的保护作用及其作用机制。方法 建立LPS诱导小鼠RAW264.7细胞体外炎症模型,采用MTT比色法测定不同浓度(160、80、40、20、10μmol/L)5-O-甲基维斯阿米醇苷对小鼠RAW264.7细胞活性的影响;实验分空白组,LPS组,阳性对照组(吲哚美辛,10μmol/L),5-O-甲基维斯阿米醇苷低(20μmol/L)、中(40μmol/L)、高(80μmol/L)剂量组,空白组、LPS组加入空白培养基,其余给药组加入相应药物,2h后加入LPS(10μg/mL),采用格里斯试剂法检测小鼠RAW264.7细胞上清液的一氧化氮(NO)的分泌,酶联免疫吸附试验法检测小鼠RAW264.7细胞中的前列腺素E_(2)(PGE_(2))、肿瘤坏死因子α(TNF-α)含量,RT-qPCR检测小鼠RAW264.7细胞核因子-κB(NF-κB)p65、白细胞介素1β(IL-1β)、诱导型一氧化氮合酶(iNOS)、环氧合酶2(COX-2)的mRNA表达,Western blot检测Toll受体4(TLR4)、NF-κB p65蛋白表达。结果5-O-甲基维斯阿米醇苷(10~80μmol/L)对小鼠RAW264.7细胞活性无明显影响。与空白组比较,LPS组小鼠RAW264.7细胞NO、PGE_(2)、TNF-α含量升高(P<0.01),NF-kB p65、IL-1β、INOS、COX-2的mRNA表达及TLR4、NF-κB p65蛋白表达增加(P<0.01);与LPS组比较,5-O甲基维斯阿米醇苷低、中、高剂量组R小鼠AW264.7细胞中NO、PGE_(2)、TNF-α含量均降低(P<0.01),NF-κB p65、IL-1β、INOS、COX-2的mRNA表达和TLR4、NF-κB p65蛋白表达均降低(P<0.01)。结论 防风中5-O甲基维斯阿米醇苷能抑制LPS诱导小鼠RAW264.7细胞炎症反应,具有一定的抗炎作用。