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.

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。

Peptide fraction from sturgeon muscle by pepsin hydrolysis exerts anti-inflammatory effects in LPS-stimulated RAW264.7 macrophages via MAPK and NF-κB pathways

Previous studies have suggested that polypeptides extracted from milk, soybean, fish, eggs, and meat possess potential anti-inflammatory effects. To date, few studies have reported the anti-inflammatory function of sturgeon peptides and their underlying mechanisms are unknown. The current study was therefore to determine the anti-inflammatory potential of sturgeon peptides with lipopolysaccharide (LPS)-induced RAW264.7 inflammatory model. Pepsin hydrolysate (PeH) was purified by ultrafiltration and Sephadex G-15 gel filtration chromatography. PeH significantly reduced the inflammatory mediator (NO) and inflammatory cytokines (IL-6, TNF-α and IL-1β) expression in a dose-dependent manner. Moreover, the purified sturgeon peptide (F2) possessed strong antioxidant potential and effectively inhibited DPPH and ABTS free radicals. F2 significantly suppressed the expression of MAPK, IκBα, and NF-κB p65, indicating that F2 exerted anti-inflammatory influence by the inhibition of MAPK and NF-κB pathways.

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.

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.

Protective effects of paeonol on LPS-induced macrophage RAW264.7 injury through TLR4/MAPK/NF-κB pathway

Objective:To study the protective effect of paeonol on LPS-induced inflammatory injury of macrophage RAW264.7 cells and its mechanism.Methods:Macrophage RAW264.7 cells were cultured and divided into blank group,LPS(1μg/mL)group,paeonol(240μmol/mL)group and TAK242(10μmol/mL)group.The cell activity was detected by CCK8 method,the cell morphology was observed by inverted microscope,the contents of GSH and MDA in cell culture medium were determined by colorimetry,the mitochondrial membrane potential was detected by JC-1 method,the expression distribution of F4/80 and p-NF-κB protein was detected by immunofluorescence method,and the expression of TLR4/MAPK/NF-κB related pathway protein was detected by Western blotting.Results:Compared with the blank group,the cell viability induced by 1μg/mL LPS was 0.4972±0.061(P<0.01),which was close to the half inhibition rate.Compared with LPS group,the expression of p-NF-κB protein in 240μmol/mL paeonol pretreated cell group was down-regulated most significantly(P<0.01),and the expression of TLR4 protein was inhibited most significantly in 10μmol/mL TAK242 pretreated cell group.Compared with LPS group(P<0.01),the cell morphology of paeonol group recovered.Decrease MDA content and increase GSH content in cell culture medium(P<0.01),In the results of mitochondrial membrane potential,the red light of paeonol group was significantly enhanced and the green light was significantly weakened(P<0.001).The expression distribution of F4/80 and p-NF-κB protein in paeonol group decreased significantly(P<0.01),and the expressions of TLR4,p-IκB,p-p38,p-JNK and p-NF-κB protein were down-regulated(P<0.05).Conclusion:Paeonol can improve the inflammatory injury of RAW264.7 cells induced by LPS,and its mechanism may be related to TLR4/MAPK/NF-κB pathway.

暖心康通过“代谢-炎症”网络调控巨噬细胞极化对心肌梗死后小鼠心室重构的影响

目的探究暖心康(红参、毛冬青)通过“代谢-炎症”网络调控巨噬细胞极化改善心肌梗死后小鼠心室重构的作用机制。方法(1)将30只C57BL/6J雄性小鼠随机分为3组:假手术组、模型组、暖心康组(1.65 g·kg^(-1)),每组10只;采用左前降支冠状动脉结扎术复制心肌梗死小鼠模型;灌胃给药,每日1次,连续4周。采用Masson染色法检测心肌组织胶原沉积情况;超声检测小鼠心功能:左室射血分数(LVEF)、收缩末期左室前壁厚度(LVAWS)及舒张末期左室前壁厚度(LVAWD);流式细胞术检测小鼠心脏巨噬细胞分布情况;qPCR法检测心脏组织乳酸脱氢酶A(LDHA)、肉碱棕榈酰转移酶1(CPT-1)、葡萄糖转运蛋白4(GLUT4)、异柠檬酸脱氢酶(IDH)、琥珀酸脱氢酶(SDHa)mRNA表达。(2)按照1.15 g·kg^(-1)剂量给予大鼠暖心康混悬液灌胃,每日2次,持续5 d,制备暖心康含药血清。采用脂多糖(LPS)诱导RAW 264.7细胞构建促炎型巨噬细胞模型。细胞分组:空白血清对照组(含5%空白血清+5%胎牛血清的培养基)、暖心康含药血清组(含5%暖心康含药血清+5%胎牛血清的培养基)、脂多糖组(含5%空白血清+5%胎牛血清的培养基+200μg·mL^(-1)脂多糖)、暖心康含药血清+脂多糖组(含5%暖心康含药血清+5%胎牛血清的培养基+200μg·mL^(-1)脂多糖),干预16 h。采用糖酵解压力测试实验检测RAW 264.7细胞糖酵解水平;qPCR法检测RAW 264.7细胞线粒体丙酮酸转运载体(MPC1)mRNA表达;MitoSox Red荧光染色法检测RAW 264.7细胞线粒体氧化应激损伤程度。结果(1)与假手术组比较,模型组小鼠的心脏胶原纤维蓝染面积明显增加,并伴有室壁变薄,左心室腔增大;LVEF、LVAWS、LVAWD等心功能指标水平均显著降低(P<0.01,P<0.001);小鼠心脏组织中LDHA、CPT-1 mRNA表达明显上调(P<0.05),GLUT4、IDH、SDHa mRNA表达显著下调(P<0.05,P<0.01),CD86染色阳性细胞数量显著增加(P<0.001)。与模型组比较,暖心康组小鼠的心脏胶原纤维沉积明显减少,且室壁厚度增加;LVEF、LVAWS、LVAWD等心功能指标水平均显著升高(P<0.05,P<0.01,P<0.001);小鼠心脏组织中LDHA、CPT-1 mRNA表达显著下调(P<0.01,P<0.001),GLUT4、SDHa、IDH mRNA表达显著上调(P<0.01),CD86阳性细胞数量显著减少(P<0.001)。(2)与空白血清对照组比较,暖心康含药血清组巨噬细胞的糖酵解水平、ROS水平均无明显变化(P>0.05),而脂多糖组巨噬细胞的糖酵解水平、ROS水平均显著升高(P<0.01),MPC1 mRNA表达显著下调(P<0.001)。与脂多糖组比较,暖心康含药血清+脂多糖组的巨噬细胞糖酵解水平、ROS水平均显著降低(P<0.05,P<0.01),MPC1 mRNA表达显著上调(P<0.001)。结论暖心康能够减轻小鼠心肌梗死后的心肌纤维化及心室重构,改善心功能,其作用机制可能与下调心脏组织LDHA mRNA表达,上调GLUT4 mRNA表达,改善心肌梗死后心脏葡萄糖摄取能力,抑制促炎型巨噬细胞糖酵解,增加SDHa及IDH的表达以减轻琥珀酸与柠檬酸堆积,减少活性氧(ROS)生成,从而减少促炎型巨噬细胞过度极化有关。

刺糖多糖调控Toll样受体4对免疫抑制活性的影响

揭示刺糖多糖对Toll样受体4(Toll-like receptor 4,TLR4)的调控机制。构建C57BL/6J免疫抑制小鼠模型及TAK-242抑制剂诱导的RAW 264.7模型,小鼠模型给予刺糖多糖组800 mg/kg以及RAW 264.7模型给予不同浓度的刺糖多糖(25、50、75、100μg/mL)进行干预。酶联免疫吸附测定法(enzyme-linked immunosorbent assay,ELISA)分别测定小鼠血清中细胞因子、RAW 264.7细胞因子分泌水平。蛋白免疫印迹(Western blot)与实时荧光定量PCR(real-time quantitative PCR,qRT-PCR)法检测TLR4和髓样分化因子88(myeloiddifferentiationfactor88,MyD88)与肿瘤坏死因子相关的分子6(TNF receptor associated factor 6,TRAF6)在相关组织和细胞中的表达。结果表明刺糖多糖显著提高了免疫抑制小鼠的脾脏指数、胸腺指数,以及血清中白细胞介素-2(interleukin-2,IL-2)、白细胞介素-4(interleukin-4,IL-4)、肿瘤坏死因子α(tumor necrosis factor-α,TNF-α)、免疫球蛋白G(Immunoglobulin G,IgG)和免疫球蛋白M(Immunoglobulin M,IgM)的含量。在TAK-242抑制剂诱导的细胞模型中,刺糖多糖增加了白细胞介素-1β(Interleukin-1β,IL-1β)、白细胞介素-6(Interleukin-6,IL-6)、白细胞介素-12(interleukin-12,IL-12)、TNF-α、核因子κB(nuclear factor-κB,NF-κB)的分泌。此外,刺糖多糖逆转了TLR4和MyD88/TRAF6的表达下调。刺糖多糖可以通过调节MyD88途径激活TLR4受体的免疫应答。

塞来昔布对脂多糖诱导的RAW264.7巨噬细胞炎症模型炎症因子的影响

目的建立脂多糖(LPS)诱导的RAW 264.7巨噬细胞炎症模型,探讨塞来昔布对其分泌炎症因子的影响。方法培养小鼠RAW 264.7巨噬细胞,采用1μg/ml的LPS刺激小鼠RAW 264.7巨噬细胞24 h后,收集细胞培养基,采用Griess法测定一氧化氮(NO)及ELISA法测定肿瘤坏死因子α(TNF-α)、前列腺素E_2(PGE_2)的含量,从而建立LPS诱导的RAW 264.7巨噬细胞炎症模型。采用MTT法检测塞来昔布对LPS刺激的RAW 264.7巨噬细胞的毒性作用后,选用8.00μmol/L塞来昔布预处理细胞1 h,再加入1μg/ml LPS刺激细胞24 h,收集细胞培养基,测定培养基中炎症因子NO、TNF-α及PGE_2的含量。结果 1μg/ml的LPS刺激RAW 264.7巨噬细胞24 h后,细胞形态出现明显变形,细胞培养基中炎症因子NO及TNF-α、PGE_2含量均较正常对照组明显增高(P<0.01)。与DMSO溶剂对照组相比,8.00μmol/L塞来昔布组能明显抑制LPS诱导的RAW 264.7巨噬细胞炎性因子NO、TNF-α及PGE_2的释放(均P<0.01)。结论成功建立LPS诱导的RAW 264.7巨噬细胞炎症模型,塞来昔布可明显抑制其炎症因子NO、TNF-α及PGE_2的分泌。

荞麦多肽对RAW 264.7细胞氧化损伤的保护作用

为提高荞麦蛋白生物利用度,利用Sephadex G-25凝胶层析和反向高效液相色谱(RP-HPLC)分离制备荞麦抗氧化多肽(BAPs),对其结构进行表征。通过H_(2)O_(2)诱导RAW 264.7巨噬细胞建立氧化应激模型,评价BAPs对细胞氧化损伤的保护作用。结果表明:经分离纯化得到的BAPs纯度达96.25%,其分子质量为5.8 ku。BAPs对DPPH·、ABTS+·、·OH清除能力及BAPs的还原力以VC当量抗氧化能力(VCEAC)分别表示为(12.12±0.27),(153.82±5.04),(901.95±39.30),(109.23±1.18)μg/mg。在细胞试验中,BAPs质量浓度达200μg/mL时,相较于模型组,对所有测定抗氧化指标均产生显著性(P<0.05)影响,细胞存活率显著提高13.80%,细胞内活性氧(ROS)水平下降40.63%,丙二醛(MDA)含量下降11.92 nmol/mg prog,超氧化物歧化酶(SOD)活力和过氧化氢酶(CAT)活力分别提高23.48 U/mg prot 15.71 U/mg prot。BAPs能有效抵抗RAW 264.7细胞产生的氧化应激反应,为开发荞麦多肽为天然抗氧化剂提供理论依据。

白藜芦醇抑制脂多糖诱导破骨前体细胞Raw264.7的激活

目的探讨白藜芦醇(Res)对脂多糖(LPS)诱导的破骨前体细胞Raw 264.7细胞系释放炎性细胞因子的抑制作用。方法采用LPS刺激Raw 264.7细胞构建炎症模型,采用抗酒石酸酸性磷酸酶(TRAP)染色鉴定细胞,采用MTT检测Res对Raw 264.7细胞的毒性影响,免疫荧光双标以及反转录聚合酶链反应(RT-PCR)方法检测不同浓度Res(1μmol/L和5μmol/L)对细胞炎性因子:肿瘤坏死因子-α(TNF-α)和白细胞介素-1β(IL-1β)与细胞炎性蛋白酶:诱导型一氧化氮合酶(i NOS)和环氧合酶-2(COX-2)、炎性信号蛋白核因子-κB(NF-κB)蛋白与mRNA的表达变化。结果不同浓度的Res(1μmol/L和5μmol/L)在翻译水平和转录水平上明显抑制了LPS诱导的细胞炎性蛋白酶i NOS和COX-2表达,同时了抑制细胞炎性因子IL-1β与炎性信号蛋白NF-κB的上调。结论 Res可能通过NF-κB调控LPS诱导的Raw 264.7细胞炎性细胞因子的释放进而抑制破骨前体细胞的激活,进而具有抗骨质疏松的作用。

核桃蛋白抗炎成分的筛选及其活性比较

研究核桃蛋白中最具有抗炎活性的组分及胃肠消化对其性质和抗炎活性的影响。利用LPS诱导的小鼠巨噬细胞RAW 264.7模型,研究6种核桃蛋白酶解物的抗炎活性;利用超滤技术将抗炎活性最强的酶解物进行分级提取,研究不同分子量超滤组分的抗炎活性;建立体外模拟胃肠消化模型,评价体外模拟消化对活性最好组分水解度、多肽含量和抗炎活性的影响。研究发现,6种蛋白酶酶解物均可抑制LPS诱导的RAW 264.7巨噬细胞的NO释放,其中碱性蛋白酶酶解物抑制效果最好,当其剂量为800μg/mL时NO释放抑制率为18.33%;碱性蛋白酶酶解物中,分子量<1 ku组分对NO释放抑制效果最好,当其剂量为800μg/mL时NO释放抑制率为25.25%;与未消化组相比,<1 ku胃肠模拟消化组的多肽含量从5.56 g/100 g增加到10.93 g/100 g,水解度从1.82%增加到7.54%,NO释放抑制率从24.75%增加到46.50%。结果表明,核桃碱性蛋白酶解物中,分子量<1 ku组分具有最强的抗炎活性,经胃肠消化后其抗炎活性增加。研究结果可为核桃抗炎肽分离纯化的研究奠定基础,也为核桃副产物高值化利用提供理论依据。

牛磺鹅去氧胆酸对小鼠巨噬细胞系RAW264.7细胞凋亡的影响

为了探讨牛磺鹅去氧胆酸(TCDCA)对小鼠单核巨噬细胞系RAW264.7的抗凋亡作用,试验采用二苯胺法及实时荧光定量PCR技术分别检测了针对RAW264.7细胞凋亡百分率及凋亡抑制蛋白CIAP-1、CIAP-2和XIAP的mRNA表达影响。结果显示,剂量为0.05、0.10和10μg/mL TCDCA可以极显著地对抗地塞米松(DEX)诱导的RAW264.7细胞系凋亡(P<0.01)。1μg/mL TCDCA对正常RAW264.7细胞系CIAP-1和XIAP表达有显著的促进作用(P<0.05);10μg/mL TCDCA对正常RAW264.7细胞系CIAP-1、CIAP-2和XIAP表达均具有显著的促进作用(P<0.05)。TCDCA给药后对DEX诱导的RAW264.7细胞系CIAP-1、CIAP-2和XIAP表达均具有极显著的促进作用(P<0.01),但不同给药剂量的TCDCA作用有所差异。以上研究结果表明,TCDCA具有对抗DEX诱导的小鼠巨噬细胞系RAW264.7凋亡作用,且与上调凋亡抑制蛋白mRNA表达有关。

脂多糖对Raw264.7巨噬细胞线粒体功能的作用效应

目的探讨脂多糖(LPS)对Raw264.7巨噬细胞线粒体内参与重要代谢途径过程中关键物质的影响。方法2020年9月—2021年2月于武汉大学第一临床学院中心实验室进行实验。体外培养小鼠Raw264.7巨噬细胞,随机分为4组,空白对照组巨噬细胞不做其他处理;脂多糖模拟机体在炎性反应过程中产生的刺激物质,分为低剂量LPS组(1μg/ml)、中剂量LPS组(5μg/ml)和高剂量LPS组(10μg/ml)。检测并比较4组细胞内线粒体呼吸链复合体Ⅰ~Ⅲ活性、异柠檬酸脱氢酶(IDH1)的活性与含量以及乳酸含量。结果与空白对照组比较,低、中、高剂量LPS组Raw264.7细胞内线粒体呼吸链复合体Ⅰ~Ⅲ活性均依次降低(F=139.363、95.123、86.795,P均<0.01),异柠檬酸脱氢酶蛋白活性、含量、相对荧光值依次降低(F=240.796、624.261、278.540,P均<0.01);乳酸含量依次升高(F=55.987,P<0.01)。结论脂多糖可抑制Raw264.7细胞内线粒体呼吸链复合体Ⅰ~Ⅲ活性、异柠檬酸脱氢酶活性及蛋白表达含量,增加Raw264.7细胞内乳酸含量,且LPS浓度越高,细胞内线粒体关键酶活性越低,乳酸含量越高。

Transcriptomic analysis reveals the effect of the exopolysaccharide of Psychrobacter sp.B-3 on gene expression in RAW264.7 macrophage cells

B-3 exopolysaccharide is extracted from the Antarctic psychrophilic bacterium Psychrobacter sp. B-3. We have previously shown that it activates macrophages and affects their immunoregulatory activities. To determine what genes are affected during this process, we detected the genes differentially expressed in cells of RAW264.7 macrophages treated with B-3 exopolysaccharide by transcriptomic analysis. B-3 exopolysaccharide treatment caused differential expression of 420 genes, of which 178 were up-regulated and 242 were down-regulated. These genes were shown to be involved in many aspects of cell function, mainly metabolism and immunity. Genes were enriched in multiple immune-related pathways, and the most significantly enriched genes were involved in antigen processing and presentation pathways. The pathway in which differentially expressed genes were the most significantly enriched was the metabolic pathway; specifically, the expression of many metabolic enzyme genes was altered by B-3 exopolysaccharide treatment. Additionally, the genes involved in metabolisms of amino acids, carbohydrates, lipids and nucleotides, varied to certain degrees. B-3 exopolysaccharide, therefore, appears to directly affect the immune function of RAW264.7 macrophages as an immunostimulant, or to indirectly change intracellular metabolism. This is the first study to determine the effect of an Antarctic psychrophilic bacterial exopolysaccharide on RAW264.7 macrophages. Our findings provide an important reference for research into the regulation of macrophage immune function by different polysaccharides.

Anti Inflammatory Property of PDRN—An <i>in Vitro</i>Study on Cultured Macrophages

Skin aging and most age-related diseases are associated with a low-grade chronic inflammation. The nucleoside adenosine, a potent endogenous anti-inflammatory agent, is deeply involved in inflammatory diseases and, by interaction with the adenosine A2 receptor (A2AR) it immediately promotes a mechanism of defence against the inflammatory damage. The aim of our study was to investigate whether polydeoxyribonucleotide (PDRN), a mixture of deoxyribonucleotides polymers of different lengths that like adenosine, binds the A2A receptor, can reduce the inflammatory state in the macrophage cell line. RAW264.7, murine macrophage cells, were incubated with PDRN in the presence and in the absence of lipopolysaccaride (LPS), which was the major component of the outer membrane of gram-negative bacteria and which acted as a strong macrophage activator. We assessed the production of nitric oxide and the secretion of inflammatory mediators (i.e., TNF-α, IL-10, IL-12 and VEGF-A). Our data showed that PDRN produced a significant decrease of inflammation in macrophages pre-stimulated with LPS, assessed in terms of the nitric oxide content (p 2A receptor, contributed to a great extent towards reducing inflammation.

Inflammatory mediator release by Brugia malayi from macrophages of susceptible host Mastomys coucha and THP-1 and RAW 264.7 cell lines

Objective:To investigate which life stage of the parasite has the ability to stimulate release of pro- or anti-inflammatory mediators from macrophages.Methods:The human macrophage/ monocyte cell line THP-1,the mouse macrophage cell line RAW 264.7 and naive peritoneal macrophages（PM） from the rodent host Mastomys coucha（M.coucha） were incubated at 37℃in 5%CO2 atmosphere with extracts of microfilariae（Mf）,third stage infective larvae（L3） and adult worms（Ad） of Brugia malayi.After 48 hr post exposure,IL-1β,IL-6,TNF-α,IL-10 and nitric oxide（NO） in cell-free supernatants were estimated.Results:Extracts of all the life stages of the parasite were capable of stimulating pro-（IL-1β,IL-6 and TNF-α） and anti-inflammatory （IL-10） cytokines in both the cell lines and peritoneal macrophages of M.coucha.Mf was the strongest stimulator of pro-inflammatory cytokines followed by L3 and Ad;however,Ad was a strong stimulator of IL-10 release.Mf was found to have potential to modulate LPS-induced NO release in RAW cells.Ad-induced NO release was concentration dependent with maximum at 20μg/mL in both RAW and PMs.Conclusions:The results show that parasites at all life stages were capable of stimulating pro-（IL-1β,IL-6 and TNF-α） and anti-inflammatory（IL-10） cytokines and NO release from macrophages of susceptible host M.coucha,human and mouse macrophage cell lines.Mf can suppress the LPS-induced NO release in RAW cells.The findings also show that the two cell lines may provide a convenient in vitro system for assaying parasite-induced inflammatory mediator release.

Stir-Fry Chicken with Green Curry Suppresses Inflammatory Gene Expression by Lipopolysaccharide-Induced Murine Macrophages

Inflammatory mediators produced during inflammatory response play an important role on pathological development of several chronic diseases. Although several dietary plants exhibited anti-inflammatory property, their impacts as a whole food has been rarely reported. The aim of the present study is to assess anti-inflammatory activity of an ethanol extract from a whole food namely “ready to eat stir-fry chicken with green curry” consisting of green curry paste, big egg plant, pea egg plant, red chili, kaffer lime and sweet basil as plant-based ingredients. The food extract at 55 - 220 μg/ml was incubated with RAW264.7 murine macrophage cells prior to stimulation with lipopolysaccharide (LPS) for 24 h. Inflammatory mediators [(inducible nitric oxide synthase (iNOS), cyclooxygenase-2 (COX-2), tumor necrosis factor (TNF-α) and interleukine-6 (IL-6)] mRNA and protein were determined by RT-PCR, immunoblot and ELISA respectively. The modulation mechanism by the food extract was observed by measuring the phosphorylated form of mitogen activated protein kinases (MAPKs) and inhibitor kappa B alpha (IκB-α). The ready to eat stir-fry chicken with green curry extract significantly suppressed LPS-induced iNOS, COX-2, IL-6 and TNF-α gene expression in a dose-depend- ent manner without cytotoxicity. The suppressive effect was modulated partly by inhibiting phosphorylation of MAPKs and IκB-α. These results indicate that spices and vegetables in a complex diet still possess strong anti-inflammatory activities which warrant confirming such activities to ameliorate the pathogenesis of inflammatory-associated chronic diseases in vivo.

结核分枝杆菌Rv1048c基因异源表达菌株的构建及其对小鼠巨噬细胞存活率的影响研究

目的对结核分枝杆菌H37Rv菌株中功能未知基因Rv1048c进行生物信息学分析,构建重组表达菌株MS_Rv1048c,并研究其对小鼠巨噬细胞存活率的影响。方法软件在线分析Rv1048c的氨基酸序列及其编码蛋白的基本性质,利用PCR扩增Rv1048c目的片段,构建重组质粒pMV261-Rv1048c,转入耻垢分枝杆菌,构建重组菌株MS_Rv1048c与空载菌MS_vec。分析该基因对菌株生长的影响;通过CCK-8、总胆固醇测定和油红(O)染色的方法,初步探究重组菌株感染巨噬细胞后对其活性的影响。结果Rv1048c基因全长1116 bp,蛋白由371个氨基酸构成,分子式是C_(1778)H_(2821)N_(521)O_(525)S_(10),预测该蛋白是一种定位在细胞外的含有多个磷酸化位点的、不稳定的亲水性蛋白。本试验首次成功构建未知基因Rv1048c的异源表达载体,生长曲线测定发现该基因使菌株生长缓慢,细胞实验发现基因增强了重组菌株对细胞的侵袭能力。结论Rv1048c可能具有结核分枝杆菌独有的生长特性,并降低在菌株侵染下的细胞的存活率。分析Rv1048c未知基因和构建异源表达菌株,有助于后续对结核分枝杆菌Rv1048c基因功能的探究,为进一步解析结核分枝杆菌的致病机制奠定了基础。

不消化性葡聚糖体外酵解液对RAW 264.7巨噬细胞的免疫调节作用

为探究不消化性葡聚糖(indigestible glucans,IGs)体外肠道菌酵解液的免疫调节活性,采用厌氧发酵模型利用健康人体粪便菌群分别对6种IGs(大麦β-葡聚糖、海带多糖、酵母β-葡聚糖、茯苓多糖、抗性淀粉和聚葡萄糖)进行24 h体外酵解,除菌过滤获得IGs酵解液,对pH值和短链脂肪酸含量进行测定。并以RAW 264.7巨噬细胞为研究对象,分为正常组、阳性组和IGs酵解液组,采用CCK-8试剂盒测定细胞活力,一氧化氮(nitric oxide,NO)检测试剂盒测定细胞NO释放量,流式细胞仪检测细胞活性氧(reactive oxygen species,ROS)含量,酶联免疫吸附测定法测定细胞因子分泌量。结果表明,相比于正常组,6种IGs的24 h酵解液均显著提高了RAW 264.7巨噬细胞活力、NO释放量、ROS产生量和小鼠肿瘤坏死因子α分泌量。各IGs 24 h肠道菌酵解液对RAW 264.7巨噬细胞均具有免疫调节的作用。