肾上腺素对THP-1巨噬细胞TGF-β1、SR-A1和CD36表达的影响

目的:探讨肾上腺素对THP-1巨噬细胞TGF-β1、SR-A1和CD36表达的影响。方法:不同浓度肾上腺素处理THP-1巨噬细胞24h,运用逆转录多聚酶链反应检测其TGF-β1、SR-A1和CD36的mRNA表达,酶联免疫吸附试验检测TGF-β1蛋白的表达,Westem-blotting检测SR-A1蛋白的表达。结果:100nmol/L及1μmol/L的肾上腺素作用THP-1巨噬细胞,引起TGF-β1 mR- NA和蛋白表达下调(p<0.05),SR-A1 mRNA和蛋白表达上调(P<0.05),1pmol/L～1μmol/L的肾上腺素处理后,各组CD36 mRNA水平无显著性变化(p>0.05)。结论:应激浓度的肾上腺素可能通过影响TGF-β1和SR-A1的表达而参与和/或促进AS的发生发展。     

佛手苷内酯对磷酸三钙磨损颗粒诱导骨细胞损伤的影响及机制*

目的:研究佛手苷内酯(BP)对磷酸三钙(TCP)磨损颗粒诱导骨细胞损伤的影响,并阐明其可能作用机制。方法:将TCP磨损颗粒与小鼠骨细胞MLO-Y4细胞共孵育48 h建立骨细胞体外损伤模型,随机分为正常对照(Control)组、TCP磨损颗粒(TCP,0.1 mg/ml)组、佛手苷内酯(1 μmol/L)组、佛手苷内酯(5 μmol/L)组和佛手苷内酯(20 μmol/L)组。MTT法和Calcein-AM染色检测各组骨细胞活性和形态改变;Hoechst 33342染色和流式细胞术分析各组骨细胞凋亡情况;实时荧光定量PCR检测各组骨细胞特征蛋白牙本质基质蛋白-1(DMP-1)、骨硬化蛋白(SOST)、成纤维细胞生长因子23(FGF23)的mRNA水平;Western blot法检测各组骨细胞中内质网应激标志蛋白葡萄糖调节蛋白78(GRP78)、蛋白激酶R样内质网激酶(PERK)、磷酸化PERK(p-PERK)、真核细胞翻译起始因子2α (eIF2α)、磷酸化eIF2α(p-eIF2α)、活性转录因子(ATF4)和 C/EBP 同源蛋白(CHOP)等的表达及caspase-3的活化变化。结果:与Control组比较,TCP组骨细胞的活性和DMP-1的mRNA水平显著降低(P＜0.05),骨细胞凋亡率及SOST、FGF23的mRNA水平显著增加(P＜0.05),GRP78、ATF4和CHOP等蛋白质表达、p-PERK/PERK值和p-eIF2α/eIF2α值显著升高;与TCP组比较,佛手苷内酯组骨细胞损伤明显减轻,骨细胞凋亡率显著减少(P＜ 0.05),GRP78、ATF4和CHOP等蛋白质表达、p-PERK/PERK值和p-eIF2α/PERK值也明显下降(P＜0.05)。结论:佛手苷内酯可明显抑制TCP磨损颗粒所致的骨细胞损伤,其机制可能与减弱TCP磨损颗粒诱导的内质网应激反应及PERK通路的活化密切相关。     

人参皂苷Rb1调节脑微血管NOS/NO改善脑细胞膜通透性

目的:探究人参皂苷Rb1在脂多糖(LPS)诱导的人脑微血管细胞模型中对脑细胞膜通透性的影响。方法:采用噻唑蓝比色法(MTT)及乳酸脱氢酶(LDH)释放检测不同浓度人参皂苷Rb1对LPS刺激人脑微血管内皮细胞系(HBMEC)存活率的影响;采用EVOM法检测HBMEC细胞通透性;采用Griess法、ELISA法及DAF-FM DA荧光探针分别检测NO、ONOO~-含量及eNOS、iNOS活性;Western blot法检测p-eNOS(ser1177)、iNOS蛋白的表达水平。结果:与正常对照组比较,LPS(5μg/m L)可明显降低HBMEC细胞存活率(P0.01);与LPS组比较,随着人参皂苷Rb1浓度的增加细胞存活率明显升高,且中、高剂量组(40、80μmol/L)具有显著性差异(P0.05、P0.01);LPS导致HBMEC单层细胞电阻值明显降低(P0.01),人参皂苷Rb1高剂量组(80μmol/L)可显著抑制LPS所致的细胞膜通透性升高(P0.05);LPS可明显降低HBMEC细胞NO含量(P0.01)升高ONOO~-含量(P0.05),人参皂苷Rb1中、高剂量组(40、80μmol/L)较LPS组具有显著升高NO含量,降低ONOO~-含量的作用(P0.05);与正常对照组比较,LPS组可明显降低HBMEC细胞磷酸化eNOS (ser1177)蛋白的表达水平,而显著升高iNOS蛋白表达水平(P0.01)。人参皂苷Rb1高剂量组(80μmol/L)较LPS组可显著升高p-eNOS(ser1177)蛋白的表达水平,降低iNOS蛋白的表达水平(P0.05)。结论:人参皂苷Rb1可有效降低iNOS活性,升高eNOS活性继而减少NO水平及ONOO~-含量,显著降低LPS导致的脑细胞膜通透性升高。     

即早基因c-fos在THP-1单核巨噬细胞亚型极化中的差异表达*

目的:探讨即早基因c-fos在THP-1巨噬细胞亚型极化过程中的表达变化。方法:运用PMA刺激诱导THP-1单核细胞极化为巨噬细胞,观察c-fos在单核细胞极化过程中的表达变化;在PMA刺激的基础上,分别运用LPS和IL-4诱导THP-1巨噬细胞向M1及M2亚型极化,实时定量PCR及Western blot技术分析刺激24 h时,细胞亚型标记物CD274、CD86和CD163的表达变化,并动态观察诱导极化过程中,c-fos的表达情况。结果:c-fos在PMA刺激THP-1单核细胞分化为巨噬细胞过程中蛋白和mRNA水平显示上调;LPS诱导THP-1巨噬细胞极化为M1型过程中,c-fos蛋白和mRNA水平表达降低,其特异性标记物在24 h呈现出M1型极化的特点(CD86蛋白表达升高,CD274、CD163蛋白表达降低);IL-4诱导THP-1巨噬细胞极化为M2型过程中,c-fos蛋白和mRNA水平表达升高,其特异性标记物在24 h表现出M2型极化的特点(CD86蛋白表达降低,CD274、CD163蛋白表达升高)。结论:c-fos参与了THP-1单核细胞向巨噬细胞极化的过程,并且可能通过抑制巨噬细胞M1亚型形成,促进巨噬细胞向M2亚型极化的作用参与巨噬细胞的亚型极化及其功能调节中。     

黄芩素抑制人巨细胞病毒感染星形胶质细胞的实验研究

目前对人巨细胞病毒(human cytomegalovirous,HCMV)感染尚无特异有效的治疗和预防手段,研究通过观察黄芩素(baicalein,BAI)抑制HCMV体外感染人星形胶质细胞引起的IE、pp65 mRNA及蛋白表达的变化,探讨黄芩素抗HCMV感染的机制。运用MTT法检测BAI组、HCMV组、HCMV+BAI组和对照组细胞的细胞活性,观察BAI对HCMV感染致人星形胶质细胞增殖异常的抑制作用;Real-time PCR检测不同组之间IE、pp65 mRNA表达的变化;免疫荧光、Western blot技术检测IE、pp65蛋白表达的变化。MTT结果显示,20μmol/L BAI+HCMV组的吸光值在24、48、72 h均高于HCMV组(P0.05);形态学观察病毒感染48 h时,HCMV组细胞出现明显的细胞病变效应(CPE),而20μmol/L BAI+HCMV组细胞状态较好,CPE不明显;Real-time PCR结果显示在感染48和72 h时20μmol/L BAI+HCMV组IE、pp65的mRNA表达明显低于HCMV组(P0.05);免疫荧光、Western blot结果显示20μmol/L BAI+HCMV组细胞的IE、pp65蛋白表达明显低于HCMV组(P0.05)。以上结果显示,适当浓度的黄芩素能抑制HCMV感染所致的细胞增殖异常,同时降低IE及pp65的mRNA和蛋白表达量。     

白术内酯Ⅱ逆转M2型巨噬细胞极化调控PDL1表达抑制A549细胞迁移

探究白术内酯Ⅱ(atractylenolideⅡ,AT-Ⅱ)对M2型巨噬细胞极化与A549细胞迁移能力的影响,并分析其潜在机制。利用PMA将THP-1细胞诱导成M0巨噬细胞,然后加入IL-4和IL-13继续诱导为M2型巨噬细胞。利用Transwell小室将M2型巨噬细胞与A549细胞共培养,分别给予0、2.5、5μmol/L的AT-Ⅱ进行作用。采用MTT实验测定共培养条件下AT-Ⅱ对A549细胞活力的影响;采用Real-time PCR检测M2型巨噬细胞Arg-1的mRNA表达水平;采用ELISA检测共培养体系中TNF-α、IL-1β的含量;采用WB检测A549细胞TLR4、p-p65、NF-κB(p65)、PDL1的蛋白表达水平;采用划痕实验检测A549细胞的迁移能力。结果显示,共培养条件下,与对照组相比,实验组(2.5、5μmol/L)A549细胞活力降低(2.5μmol/L组P>0.05、5μmol/L组P<0.01);M2型巨噬细胞特异性基因Arg-1的mRNA表达水平显著降低(P<0.01);M1型巨噬细胞相关炎性因子TNF-α、IL-1β含量增多但无显著差...     

冠蛋白-1不同表达水平对巨噬细胞iNOS、TLRs表达以及凋亡的影响

冠蛋白-1(Coronin-1)在真核细胞中广泛表达,涉及钙离子稳态、细胞骨架动力学、免疫及炎症反应等多种细胞功能。该研究探讨了冠蛋白-1不同表达水平对巨噬细胞诱导性一氧化氮合酶(inducible nitric oxide synthase,iNOS)、Toll样受体(Toll-like receptors,TLRs)表达和凋亡的影响并探讨其分子机制。根据冠蛋白-1表达水平的差异,实验细胞分为RAW264.7-Cor.Plus、RAW264.7、RAW264.7-Cor.Minus 3组。各组细胞分别经4μmol/L钙调磷酸酶抑制剂环孢素A(cyclosporin A,Cs A)处理24 h或2μmol/L肌动蛋白聚合抑制剂松胞菌素D(cytochalasin D,cyt D)处理48 h,同时设未处理对照,再分别用Real-time PCR法检测iNOS m RNA水平,Western blot法检测细胞TLR2、TLR4、TLR9及钙调磷酸酶(calcineurin,Ca N)的蛋白质水平,流式细胞术检测细胞凋亡百分率。各组细胞用四甲基异硫氰酸荧光素标记的鬼笔环肽(TRITC-phalloidin)染色后,计算纤维型肌动蛋白(F-actin)重排率。结果显示,冠蛋白-1过表达细胞相对于冠蛋白-1正常表达细胞,其iNOSm RNA水平以及TLR2、TLR4、TLR9蛋白表达水平和细胞凋亡率均显著降低(P0.05);Cs A作用后,RAW264.7-Cor.Plus的iNOS m RNA水平以及TLR2、TLR4、TLR9蛋白质水平和细胞凋亡率均较未处理对照细胞显著增加(P0.05),RAW264.7和RAW264.7-Cor.Plus细胞的Ca N水平较未处理对照细胞显著降低(P0.05);cyt D作用后,与未处理对照细胞相比,iNOS m RNA水平及细胞凋亡率无显著性差异(P0.05),但TLRs的表达显著降低(P0.05);经鬼笔环肽染色后,RAW264.7-Cor.Plus细胞F-actin重排率显著高于RAW264.7细胞(P0.05)。以上结果表明,冠蛋白-1过表达不仅促进了巨噬细胞F-actin重排,而且下调了iNOS、TLRs水平并且抑制细胞凋亡,其分子机制与冠蛋白-1促进钙调磷酸酶调控的Ca~(2+)信号通路有关。     

肌动蛋白解聚对巨噬细胞TLRs的表达及细胞凋亡的影响

在肺癌等的癌细胞中,脂多糖(lipopolysaccharide, LPS)等致炎因子介导的促瘤效应涉及Toll样受体(Toll like receptors, TLRs)/纤维型肌动蛋白(fibrous actin, F-actin)通路。该研究探讨了外源性松胞菌素D(cytochalasin D, cytD)和细胞内源过表达的重组肌动蛋白解聚因子丝切蛋白(Cofilin-1)所诱导的肌动蛋白解聚对巨噬细胞TLR2、TLR4和TLR9的表达和细胞凋亡水平的影响。分别用6种不同浓度的cytD处理RAW264.7小鼠巨噬细胞48 h,用Western blot检测6组细胞TLR2、TLR4、TLR9的表达水平。构建重组pEGFP-N1-Cofilin-1质粒并转染RAW264.7细胞,设置空质粒对照和空白细胞对照组。用Real-time PCR法和Western blot检测细胞转染前后Cofilin-1表达水平;Western blot检测巨噬细胞TLR2、TLR4、TLR9的表达情况;用流式细胞术检测3组细胞的凋亡水平。结果显示,终浓度≥1.5μmol/L的cytD处理细胞后, RAW264.7细胞表达TLR2明显降低(P0.05);终浓度≥1.0μmol/L的cytD处理细胞后,巨噬细胞表达TLR4、TLR9明显降低(P0.05)。重组质粒转染组细胞的cofilin-1 mRNA及Cofilin-1蛋白水平均高于空质粒对照组和空白细胞对照组(P0.05),且其TLR2、TLR4、TLR9蛋白表达水平和细胞凋亡水平均显著低于空质粒对照组和空白细胞对照组(P0.05)。结果表明,外源性cytD和巨噬细胞内源性高表达的Cofilin-1蛋白均可下调巨噬细胞TLR2、TLR4、TLR9的表达,其中,细胞高表达的Cofilin-1蛋白还显著降低了细胞凋亡率。该文通过揭示肌动蛋白解聚对巨噬细胞TLRs的表达及细胞凋亡的抑制,为进一步研究炎症与肿瘤的关系及分子机制奠定了基础。     

黄芪甲苷对马兜铃酸诱导的巨噬细胞M1型极化的作用及机制研究

目的:探讨黄芪甲苷对马兜铃酸诱导的RAW264.7细胞向M1型极化的影响,并初步探索其可能的作用机制.方法:分别采用马兜铃酸和脂多糖(LPS)刺激RAW264.7细胞24h,伴或不伴黄芪甲苷进行药物干预处理.采用细胞计数检测试剂盒-8(CCK8)检测细胞活性变化,流式细胞仪检测巨噬细胞分型,酶联免疫吸附试验(ELISA...     

Anti-inflammatory effect of chrysin on RAW 264.7 mouse macrophages induced with polyinosinic-polycytidylic acid

Chrysin (5,7-Dihydroxyflavone) is an active flavonoid isolated from Scutellariae Radix which has been used to treat pneumonia, laryngopharyngitis, jaundice, shigellosis, and breast mass in Korea, China, and Japan. Chrysin has been already reported to inhibit inducible nitric oxide synthase and cyclooxygenase-2 in lipopolysaccharideinduced macrophages. However, the effect of chrysin on virus-induced macrophages is not fully reported. In this study, the anti-inflammatory effect of chrysin on doublestranded RNA (dsRNA)-induced macrophages was examined. Production of Nitric oxide (NO), various cytokines, as well as calcium release and mRNA expression of CHOP and Fas in dsRNA [polyinosinic-polycytidylic acid]-induced RAW 264.7 mouse macrophages were evaluated. Chrysin restored the cell viability in dsRNA [polyinosinicpolycytidylic acid]-induced RAW 264.7 mouse macrophages at concentrations of up to 50 μM. Chrysin significantly inhibited the production of NO, IL-1α, IL-1β, IL-6, IL-10, IP-10, G-CSF, GM-CSF, LIF, LIX/CXCL5, MCP-1, MCSF, MIP-1α, MIP-1β, MIP-2, RANTES, TNF-α, and VEGF as well as calcium release and mRNA expression of CHOP and Fas in dsRNA [polyinosinic-polycytidylic acid]-induced RAW 264.7 mouse macrophages (P< 0.05). These data suggest that chrysin has anti-inflammatory properties related with its inhibition of nitric oxide, cytokines, chemokines, and growth factors in dsRNA-induced macrophages via the ER stress-CHOP pathway.     

Osteopontin is induced by nitric oxide in RAW 264.7 cells

Nitric oxide (NO) produced by macrophages is thought to contribute to various pathological conditions. Osteopontin (OPN) is a phosphorylated glycoprotein produced principally by macrophages. OPN inhibits inducible nitric oxide synthase (iNOS), which generates large amounts of NO production. However, the relationship between NO and endogenous OPN in activated macrophages has not yet been elucidated. We therefore examined expression of endogenous iNOS and OPN in a murine macrophage cell line, RAW 264.7 cells, by treating the cells with lipopolysaccharide (LPS) and interferon-gamma (IFN-gamma). Treatment of cells with LPS and IFN-gamma resulted in an increase of iNOS mRNA to maximum at 12 h after stimulation. In contrast, OPN mRNA was induced more slowly than iNOS mRNA. Induction of both iNOS and OPN mRNA in RAW 264.7 cells was markedly suppressed by addition of the specific iNOS inhibitor S-2-aminoethyl isothiourea dihydrobromide. The NOS inhibitor NG-methyl-L-arginine also suppressed induction of OPN mRNA but hardly affected iNOS mRNA expression. The NO-releasing agent spermine-NONOate but not peroxynitrite enhanced induction of OPN mRNA. These results suggest that NO directly up-regulates the endogenous OPN in macrophages stimulated with LPS and IFN-gamma. This up-regulation of endogenous OPN may represent a negative feedback system acting to reduce iNOS expression.     

Antioxidant enzymes suppress nitric oxide production through the inhibition of NF-kappa B activation: role of H(2)O(2) and nitric oxide in inducible nitric oxide synthase expression in macrophages.

Reactive molecules O(-)(2), H(2)O(2), and nitrogen monoxide (NO) are produced from macrophages following exposure to lipopolysaccharide (LPS) and involved in cellular signaling for gene expression. Experiments were carried out to determine whether these molecules regulate inducible nitric oxide synthase (iNOS) gene expression in RAW264.7 macrophages exposed to LPS. NO production was inhibited by the antioxidative enzymes catalase, horseradish peroxidase, and myeloperoxidase but not by superoxide dismutase (SOD). In contrast, the NO-producing activity of LPS-stimulated RAW264.7 cells was enhanced by the NO scavengers hemoglobin (Hb) and myoglobin. The antioxidant enzymes decreased levels of iNOS mRNA and protein in LPS-stimulated RAW264.7 cells, whereas the NOS inhibitor N(G)-monomethyl-L-arginine as well as Hb increased the level of iNOS protein but not mRNA, indicating that NO inhibits iNOS protein expression. NF-kappa B was activated in LPS-stimulated RAW264.7 cells and the activation was significantly inhibited by antioxidant enzymes, but not by Hb. Similar results were obtained using LPS-stimulated rodent peritoneal macrophages. Extracellular O(-)(2) generation by LPS-stimulated macrophages was suppressed by SOD, but not by antioxidative enzymes, while accumulation of intracellular reactive oxygen species was inhibited by antioxidative enzymes, but not by SOD. Exogenous H(2)O(2) induced NF-kappa B activation in macrophages, which was inhibited by catalase and pyrroline dithiocarbamate (PDTC). H(2)O(2) enhanced iNOS expression and NO production in peritoneal macrophages when added with interferon-gamma, and the effect of H(2)O(2) was inhibited by catalase and PDTC. These findings suggest that H(2)O(2) production from LPS-stimulated macrophages participates in the upregulation of iNOS expression via NF-kappa B activation and that NO is a negative feedback inhibitor of iNOS protein expression.     

红毛五加多糖单一组分AHP-Ⅲ对巨噬细胞的免疫调节作用及其机制

探讨红毛五加多糖(Acanthopanax giraldii Hams polysaccharide)单一组分AHP-Ⅲ(Acanthopanax giraldii Hams polysaccharideⅢ)对小鼠巨噬细胞RAW 264.7的激活作用及机制。不同浓度AHP-Ⅲ作用RAW 264.7细胞,中性红试验检测细胞吞噬能力;ELISA和Griess法检测其IL-6、TNF-α和NO的释放量;RT-qPCR检测iNOS、TNF-α和IL-6 mRNA相对表达水平;Western blot检测NF-κB信号通路相关蛋白磷酸化水平。在实验浓度范围内,AHP-Ⅲ可显著增强RAW 264.7细胞的吞噬能力(P<0.05);促进RAW 264.7分泌NO、TNF-α和IL-6(P<0.05或P<0.001);并显著增加RAW 264.7细胞中IL-6、TNF-α和iNOS mRNA的表达量,呈剂量依赖性;Western blot结果表明,AHP-Ⅲ作用RAW 264.7细胞后,NF-κB中的p65、IKKβ、IκBα磷酸化水平明显升高。结果显示红毛五加多糖AHP-Ⅲ对小鼠巨噬细胞RAW 264.7具有显著激活作用。     

Inhibitory effect of caveolin-1 on endoplasmic reticulum stress-induced apoptosis in macrophages via p38 MAPK pathway

Endoplasmic reticulum (ER) stress occurs in macrophage-rich areas of advanced atherosclerotic lesions and contributes to macrophage apoptosis and subsequent plaque necrosis. The purpose of the present study was to investigate the effects of caveolin-1 (Cav-1) on ER stress-induced apoptosis in cultured macrophages and the underlying mechanisms. RAW264.7 cells were incubated with thapsigargin (TG) to establish ER stress model. And Cav-1 expression was detected by Western blot. After being pretreated with filipin(III), a caveolae inhibitor, RAW264.7 cells were assayed with flow cytometry and confocal laser scanning microscopy to detect cell apoptosis. Moreover, p38 mitogen-activated protein kinase (MAPK) phosphorylation and C/EBP homologous protein (CHOP) expression were detected with Western blot. The results showed that Cav-1 expression was markedly increased at early stage of TG treatment (P < 0.05) and then decreased with prolonged or high dose TG treatments. The increasing of Cav-1 expression induced by TG in RAW264.7 cells was abolished under inhibition of caveolae by filipin(III) (P < 0.05). The effect of TG on apoptosis of RAW264.7 cells was further augmented after pretreatment with filipin(III) (P < 0.05). Western blotting showed that MAPK phosphorylation induced by TG was inhibited by filipin(III) in RAW264.7 cells (P < 0.05), whereas CHOP remained unchanged (P > 0.05). These results suggest that Cav-1 may play a critical role in suppressing ER stress-induced macrophages apoptosis in vitro, and one of the mechanisms may be correlated with the activation of p38 MAPK prosurvival pathway.     

流感病毒感染巨噬细胞对缺氧诱导因子-1α诱导炎症反应通路的机制研究

为探索缺氧诱导因子(hypoxia inducible factor,HIF)-1α诱导甲型流感病毒毒株感染小鼠巨噬细胞引起炎症反应的具体机制,本研究以甲型H1N1流感病毒(简称H1N1)株A/PR/8感染小鼠巨噬细胞RAW264.7后,在显微镜下观察其在感染后的表型变化,分别在不同时间段收集样本,通过聚合酶链反应(polymerase chain reaction,PCR)检测HIF-1α、干扰素(interferon,IFN)-γ、白细胞介素(interleukin,IL)-6、肿瘤坏死因子(tumor necrosis factor,TNF)-α和M蛋白(M protein,MBP)mRNA的变化,通过蛋白质印迹法(Western blot, WB)检测HIF-1α、核转录因子-κB(nuclear factor-κB,NF-κB)、促分裂原活化的蛋白激酶(mitogenactivated protein kinase,MAPK)、蛋白激酶B(protein kinase B,Akt)以及M蛋白的变化。随后,加入抑制剂2-MeOE-2(10 nmol/L)进行抑制试验,采用PCR和WB检测HIF-1α表达被抑制后上述炎症因子mRNA表达水平及炎症蛋白通路的变化。结果显示,H1N1PR8感染小鼠巨噬细胞RAW264.7后,H1N1PR8复制率在24 h达到峰值,HIF-1α mRNA在感染6 h后开始升高,12 h迅速上升,24 h达到峰值。IFN-γ、IL-6、TNF-α mRNA变化趋势基本与HIF-1α一致,但在感染12 h并未进入快速上升期。HIF-1α蛋白在感染后6 h表达明显增多,24 h达到峰值,与mRNA变化水平基本一致。NF-κB通路蛋白在感染12 h后明显增多,48 h开始减少。加入抑制剂2-MeOE-2后,培养感染细胞24 h,抑制剂组IL-6、TNF-α mRNA水平较对照组显著下降(P<0.05),抑制剂组NF-κB通路蛋白较对照组表达下降。本研究结果表明,小鼠巨噬细胞被H1N1感染后,HIF-1α可能通过激活NF-κB通路促进IL-6、TNF-α等炎症因子的分泌参与炎症反应。     

Ca2+/calmodulin-dependent protein phosphatase calcineurin mediates the expression of iNOS through IKK and NF-kappaB activity in LPS-stimulated mouse peritoneal macrophages and RAW 264.7 cells

Ca(2+) and Ca(2+)/calmodulin-dependent protein phosphatase calcineurin (CN) have been known to play crucial roles in immune response and inflammation. Using mouse peritoneal macrophages and RAW 264.7 macrophage cells, we demonstrated that LPS mobilized intracellular free Ca(2+) and induced CN phosphatase activity. iNOS expression and NO secretion in response to LPS were suppressed by Ca(2+) antagonists (TMB-8, BAPTA/AM, and nifedipine) and CN inhibitor (cyclosporin A). Transient expression of constitutively active CN in mouse peritoneal macrophages and RAW 264.7 macrophages strongly activated NF-kappaB, a key mediator of iNOS expression. We also found that CN mediates NF-kappaB activation via IkappaB-alpha hyperphosphorylation and degradation. Overexpression of dominant negative mutant of IKKalpha and -beta demonstrates that only IKKbeta is the target for CN. These results indicate that CN is required for full iNOS expression and the effective activation of NF-kappaB in RAW 264.7 and peritoneal macrophages.     

Anethum graveloens flower extracts inhibited a lipopolysaccharide-induced inflammatory response by blocking iNOS expression and NF-κB activity in macrophages

Inflammation is a system used by a host to defend against the presence of bacteria, viruses, or yeasts. Toll-like receptors (TLRs) in the plasma membranes of macrophages are activated when they recognize the molecular structure of a virus or bacterium. Lipopolysaccharide (LPS), an outer cell-wall component of Gram-negative bacteria, initiates an inflammatory process via TLR4. We investigated the effect of the extract of Anethum graveloens flowers (AGFs) on LPS-mediated inflammation in RAW 264.7 cells. The extract markedly suppressed nitric oxide generation in a concentration-dependent manner in LPS-stimulated RAW 264.7 cells. It inhibited inducible nitric oxide synthase (iNOS) and the mRNA expression of cytokines such as interleukin-1 beta and interleukin-6 in LPS-stimulated RAW 264.7 cells. It also inhibited iNOS protein levels in LPS-stimulated RAW 264.7 cells. In addition, AGF decreased the LPS-induced phosphorylation of mitogen-activated protein kinases in LPS-stimulated RAW 264.7 cells. AGF inhibited the phosphorylation of Akt, an upstream molecule of the nuclear factor kappa B (NF-κB) pathway, and thus inhibited NF-κB activity in LPS-stimulated RAW 264.7 cells. These results suggest that AGF exerts an anti-inflammatory effect in LPS-stimulated RAW 264.7 cells by inhibiting iNOS expression and blocking the NF-κB pathway.