Neuropeptide Y promotes TGF-β1 production in RAW264.7 cells by activating PI3K pathway via Y1 receptor

Objective To examine the effect of neuropeptide Y （NPY） on TGF-β1 production in RAW264.7 macrophages. Methods Enzyme linked immunosorbent assay （ELISA） was used to detect TGF-β1 production. Cell counting kit 8 （CCK-8） was used to assay the viability of RAW264.7 cells. Western blot was used to detect the phosphorylation of PI3K p85. Results NPY treatment could promote TGF-β1 production and rapid phosphorylation of PI3K p85 in RAW264.7 cells via Y1 receptor. The elevated TGF-β 1 production induced by NPY could be abolished by wortrnannin pretreatment. Conclusion NPY may elicit TGF-β production in RAW264.7 cells via Y1 receptor, and the activated PI3K pathway may account for this effect.

Neutrophil peptide 1 accelerates the clearance of degenerative axons during Wallerian degeneration by activating macrophages after peripheral nerve crush injury

Macrophages play an important role in peripheral nerve regeneration,but the specific mechanism of regeneration is still unclear.Our preliminary findings indicated that neutrophil peptide 1 is an innate immune peptide closely involved in peripheral nerve regeneration.However,the mechanism by which neutrophil peptide 1 enhances nerve regeneration remains unclear.This study was designed to investigate the relationship between neutrophil peptide 1 and macrophages in vivo and in vitro in peripheral nerve crush injury.The functions of RAW 264.7 cells we re elucidated by Cell Counting Kit-8 assay,flow cytometry,migration assays,phagocytosis assays,immunohistochemistry and enzyme-linked immunosorbent assay.Axonal debris phagocytosis was observed using the CUBIC(Clear,Unobstructed Brain/Body Imaging Cocktails and Computational analysis)optical clearing technique during Wallerian degeneration.Macrophage inflammatory factor expression in different polarization states was detected using a protein chip.The results showed that neutrophil peptide 1 promoted the prolife ration,migration and phagocytosis of macrophages,and CD206 expression on the surfa ce of macrophages,indicating M2 polarization.The axonal debris clearance rate during Wallerian degeneration was enhanced after neutrophil peptide 1 intervention.Neutrophil peptide 1 also downregulated inflammatory factors interleukin-1α,-6,-12,and tumor necrosis factor-αin invo and in vitro.Thus,the results suggest that neutrophil peptide 1 activates macrophages and accelerates Wallerian degeneration,which may be one mechanism by which neutrophil peptide 1 enhances peripheral nerve regeneration.

硫酸镁对脂多糖诱导巨噬细胞表达和释放高迁移率族蛋白1的影响

目的探讨硫酸镁对脂多糖(LPS)诱导小鼠巨噬细胞RAW264.7表达和释放高迁移率族蛋白1(HMGB1)的抑制作用。方法传代培养的小鼠RAW264.7细胞分5组接种于6孔板,每组为3孔。C组为仅加RPMI 1640培养液的对照组,LPS组为在RPMI 1640培养液的基础上加500ng/mL LPS的诱导组,M1组为在LPS组基础上加1mmol/L硫酸镁的干预组,M5组为在LPS组的基础上加5mmol/L硫酸镁的干预组,M10组为在LPS组基础上加10mmol/L硫酸镁的干预组。孵育24h后,收集细胞及细胞培养上清液,采用反转录聚合酶链反应(RT-PCR)和酶联免疫吸附试验(ELISA)分别检测各组细胞内HMGB1mRNA表达水平和细胞培养上清液中HMGB1蛋白含量的变化。结果 M1、M5、M10组的RAW264.7细胞活性分别为1.35±0.10、1.34±0.11、1.31±0.08,差异均无统计学意义(P值均>0.05)。LPS、M1、M5、M10组细胞上清液中HMGB1蛋白的含量分别为(82.80±9.15)、(81.26±8.47)、(56.69±6.21)、(50.71±6.62)ng/mL,均显著高于C组(C组为0,P值均<0.05);M5、M10组细胞上清液中HMGB1蛋白的含量均显著低于LPS及M1组(P值分别<0.05或0.01)。LPS、M1、M5、M10组细胞中HMGB1 mRNA的相对表达量分别为1.435±0.161、1.416±0.124、0.873±0.093、0.774±0.067,均显著高于C组的0.195±0.020(P值均<0.05);M5、M10组细胞中HMGB1mRNA的相对表达量均显著低于LPS及M1组(P值分别<0.05或0.01)。结论硫酸镁抑制LPS诱导的RAW264.7细胞表达和释放HMGB1,通过抑制与脓毒症致死性密切相关的关键炎性因子,可能对脓毒症患者具有一定保护作用。

低镁对脂多糖诱导巨噬细胞表达和释放高迁移率族蛋白1的影响

目的探讨低镁对脂多糖(LPS)诱导小鼠巨噬细胞RAW264.7表达和释放高迁移率族蛋白1(HMGB1)的促进作用。方法传代培养的小鼠RAW264.7细胞分为4组,接种于6孔板,每组为3孔,4组分别为含1mmol/L硫酸镁的RPMI1640培养基组(C1组)、含0.1mmol/L硫酸镁的RPMI1640培养基组(C0.1组)、含1mmol/L硫酸镁的RPMI1640培养基加500ng/mLLPS的刺激组(L1组)和含0.1mmol/L硫酸镁的RPMI1640培养基加500ng/mLLPS的刺激组(L0.1组)。孵育24h后,收集细胞及细胞培养上清液,用反转录-聚合酶链反应和酶联免疫吸附试验分别检测各组细胞内HMGB1mRNA表达水平和细胞培养上清液中HMGB1蛋白含量的变化。结果 C0.1组与C1组间HMGB1mRNA及蛋白表达的差异均无统计学意义(P值均>0.05),L1组和L0.1组HMGB1mRNA及蛋白的表达均显著高于C0.1组和C1组(P值均<0.05),L0.1组又显著高于L1组(P值均<0.05)。结论低镁促进LPS诱导的RAW264.7细胞表达和释放HMGB1,可能对脓毒症患者的预后有一定损害作用。

缺氧通过HIF-1α介导NRP-1上调抑制破骨细胞分化

目的研究低氧/HIF-1α通路对RAW264.7细胞向成熟破骨细胞分化的调控作用,并初步探讨其可能的分子机制。方法采用短发夹RNA(short hairpin RNA,shRNA)慢病毒感染法,分别建立HIF-1α和NRP-1稳定低表达的RAW264.7细胞系。将RAW264.7细胞分组培养:对照组,分化组(RANKL 100 ng/mL+50%成骨细胞CM),缺氧组(RANKL 100 ng/mL+50%成骨细胞CM+100μmol/L CoCl_2氯化钴),缺氧+HIF-1α-NC组,缺氧+HIF-1α-shRNA干扰组,缺氧+NRP-1-NC组及缺氧+NRP-1-shRNA干扰组。TRAP染色观察破骨细胞的分化情况;RT-PCR检测Cath K、MMP-9、TRAP、HIF-1α和NRP-1 mRNA的表达;Western blot检测HIF-1α和NRP-1蛋白的表达。结果①缺氧组破骨细胞分化相关基因Cath K、MMP-9、TRAP mRNA的表达量及TRAP染色阳性细胞数均明显低于分化组(P<0.05)。②缺氧组细胞中HIF-1α和NRP-1的表达均明显高于分化组(P<0.05)。③与缺氧组相比,缺氧+HIF-1α-shRNA干扰组TRAP染色阳性细胞数及破骨细胞分化相关基因的表达均明显增加(P<0.05);且HIF-1α和NRP-1表达均明显减少(P<0.05)。④与缺氧组相比,缺氧+NRP-1-shRNA干扰组TRAP染色阳性细胞数及破骨细胞分化相关基因的表达均明显增加(P<0.05);且NRP-1表达明显减少(P<0.05)。结论在RAW264.7细胞中,CoCl_2诱导的缺氧能够通过上调HIF-1α增强NRP-1的表达,从而抑制其向成熟破骨细胞分化。

脂多糖(LPS)对小鼠Raw 264.7细胞Irak1bp1表达的影响

目的研究脂多糖(lipopolysaccharide,LPS)刺激小鼠Raw264.7细胞IL-1受体相关激酶1结合蛋白1(IL-1 receptor associated kinase 1 binding protein1,Irak1bp1)的表达情况。方法体外培养的小鼠Raw264.7细胞随机分为2组:A组为正常对照组,B组为LPS刺激组。LPS刺激小鼠Raw264.7细胞6h后收集细胞及上清液。采用实时荧光定量PCR法检测IL-6及Irak1bp1mRNA水平;采用ELISA分析培养上清液中IL-6含量;采用Western blot方法检测Irak1bp1蛋白质水平。结果LPS刺激组炎症因子IL-6mRNA及蛋白质水平较对照组明显增高(P<0.01),Irak1bp1mRNA及总蛋白质水平高于对照组(P<0.05);胞质内Irak1bp1蛋白质水平与对照组相比无明显变化,而胞核内Irak1bp1蛋白质水平较正常对照组增加(P<0.01)。结论LPS能够诱导Raw264.7细胞核内Irak1bp1表达,且该分子的表达上调可能与细胞的炎性因子释放相关。

Dieckol isolated from Eisenia bicyclis extract suppresses RANKL-induced osteoclastogenesis in murine RAW 264.7 cells

Objective:To demonstrate the effect of dieckol from Eisenia bicyclis on osteoclastogenesis using RAW 264.7 cells.Methods:Murine macrophage RAW 264.7 cells were subjected to dieckol treatment,followed by treatment with receptor activator of nuclear factor kappa-B ligand(RANKL)to induce osteoclastogenesis.Tartrate-resistant acid phosphatase(TRAP)activity was examined using a TRAP activity kit.Western blotting analysis was conducted to examine the level of osteoclast-related factors,including TRAP and calcitonin receptor(CTR),transcriptional factors,including c-Fos,c-Jun,and nuclear factor of activated T cells cytoplasmic 1(NFATc1),nuclear factor kappa-B(NF-κB),extracellular signal-regulated kinase(ERK),and c-Jun N-terminal kinase(JNK).Immunofluorescence staining was conducted to examine the expression of c-Fos,c-Jun,and NFATc1.Results:Among the four phlorotannin compounds present in Eisenia bicyclis,dieckol significantly hindered osteoclast differentiation and expression of RANKL-induced TRAP and CTR.In addition,dieckol downregulated the expression levels of c-Fos,c-Jun,NFATc1,ERK,and JNK,and suppressed NF-κB signaling.Conclusions:Dieckol can suppress RANKL-induced osteoclastogenesis.Therefore,it has therapeutic potential in treating osteoclastogenesis-associated diseases.

PI3K/Akt pathway is involved in the activation of RAW 264.7 cells induced by hydroxypropyltrimethyl ammonium chloride chitosan

We previously demonstrated that 2-hydroxypropyltrimethyl ammonium chloride chitosan(HACC)promoted the production of nitric oxide(NO)and proinflammatory cytokines by activating the mitogen-activated protein kinases(MAPK)and Janus kinase(JAK)/STAT pathways in RAW 264.7 cells,indicating good immunomodulatory activity of HACC.In this study,to further investigate the immunomodulatory mechanisms of HACC,we determined the roles of phosphatidylinositol 3-kinase(PI3K)/Akt,activating protein(AP-1)and nuclear factor kappa B(NF-κB)in HACC-induced activation of RAW 264.7 cells by the western blotting.The results suggest that HACC promoted the phosphorylation of p85 and Akt.Furthermore,c-Jun and p65 were also increased after the treatment of RAW 264.7 cells with HACC,indicating the translocation of NF-κB and AP-1 from cytoplasm to nucleus.In addition,as scanning electron microscopy(SEM)analysis shows,the cell morphology changed after HACC treatment.These findings indicate that HACC activated MAPK,JAK/STAT,and PI3K/Akt signaling pathways dependent on AP-1 and NF-κB activation in RAW 264.7 cells,ultimately leading to the increase of NO and cytokines.

蛇莓乙醇提取物的体外抗炎机制研究

目的研究蛇莓乙醇提取物在体外的抗炎作用,初步探讨其抗炎机制。方法通过脂多糖(LPS)干预RAW264.7巨噬细胞系建立炎症细胞模型,ELISA法检测上清液中TNF-α、NO的分泌量,实时荧光定量RT-PCR法检测TNF-α、i NOS、血红素氧合酶-1(HO-1)的基因表达,Western blot法测定HO-1的蛋白表达量,免疫细胞化学法检验核因子-κB(NF-κB)的表达及分布变化。结果蛇莓提取物干预后细胞所分泌的炎症介质(TNF-α和NO)与炎症模型组相比均显著降低(均P<0.01),并存在剂量依赖关系;实时荧光定量RT-PCR结果显示蛇莓提取物干预后细胞TNF-α、i N-OS的mRNA表达水平显著降低,HO-1的mRNA表达水平明显升高,差异均有统计学意义,也存在剂量依赖关系;Western blot结果显示药物干预后HO-1的蛋白表达水平明显升高(P<0.01);免疫细胞化学法结果显示仅有LPS干预时,NF-κB表达增强且集中分布在细胞核,而药物干预时,NF-κB多分布在胞质。结论蛇莓提取物通过抑制NF-κB的激活,下调巨噬细胞表达炎症介质,同时促进HO-1的释放而发挥一定的抗炎作用。