Study on mechanism of increased allergenicity induced by Ara h 3 from roasted peanut using bone marrow-derived dendritic cells

Little information was so far available about allergenic mechanism of the roasted peanut allergens during initial stages of allergy.The purpose of this study was to determine the influence of roasting(150℃,20 min)on biochemical and biological properties of Ara h 3,a major peanut allergen.Allergenicity of roasted peanut emulsion to mice,differences in uptakes between Ara h 3 purified from raw peanuts(named as Ara h 3-Raw)and that purified from roasted peanuts(named as Ara h 3-Roasted)by bone marrow-derived dendritic cells(BMDCs)and the implication of cell surface receptors involving in uptake,and changes in glycosylation and structure of Ara h 3 after roasting were analyzed in this study.This study suggested that roasting increased allergenicity of peanut to BALB/c mice.Maillard reaction and structural changes of Ara h 3 induced by roasting significantly altered the uptake of Ara h 3-Roasted by BMDCs,and modified Ara h 3 fate in processes involved in immunogenicity and hyper allergenicity,indicating that food processing pattern can change food allergenicity.

The role of bone marrow-derived cells in the origin of liver cancer revealed by single-cell sequencing

Objective:Epithelial cancers often originate from progenitor cells,while the origin of hepatocellular carcinoma(HCC)is still controversial.HCC,one of the deadliest cancers,is closely linked with liver injuries and chronic inflammation,which trigger massive infiltration of bone marrow-derived cells(BMDCs)during liver repair.Methods:To address the possible roles of BMDCs in HCC origination,we established a diethylnitrosamine(DEN)-induced HCC model in bone marrow transplanted mice.Immunohistochemistry and frozen tissue immunofluorescence were used to verify DENinduced HCC in the pathology of the disease.The cellular origin of DEN-induced HCC was further studied by single cell sequencing,single-cell nested PCR,and immunofluorescence-fluorescence in situ hybridization.Results:Studies by using single cell sequencing and biochemical analysis revealed that HCC cells in these mice were coming from donor mice BMDCs,and not from recipient mice.Furthermore,the copy numbers of mouse orthologs of several HCC-related genes previously reported in human HCC were also altered in our mouse model.DEN-induced HCCs exhibited a similar histological phenotype and genomic profile as human HCCs.Conclusions:These results suggested that BMDCs are an important origin of HCC,which provide important clues to HCC prevention,detection,and treatments.

Recombinant E.coli LLO/OVA Induces Murine BMDCs Maturation via TLR4 and NOD1 Receptor and Promotes Specific Cytotoxic T Cell Immunity

Objective To explore the immune stimulation effect of recombinant E.coli LLO/OVA on mice bone marrow-derived dendritic cells （BMDCs） and T lymphocytes in vitro.Methods After BMDCs stimulated by E.coli LLO/OVA,their Toll-like receptor （TLR） and nucleotide-binding oligomerization domain （NOD） receptor signalling pathway were examined by superarray hybridization;and the priming effect of the vaccine activated BMDCs on CD4＋T and CD8＋T was determined by [3H]thymidine uptake and ELISA,the tumor cytotoxic effect of activated CD8＋T cells was determined by cytotoxic assay.Results After BMDCs were activated by E.coli LLO/OVA via TLR4,NOD1 receptor and NF-κB signalling pathway,the expression of their surface molecules including MHC class Ⅰ,MHC class Ⅱ,CD40,CD80 and CD86 significantly up-regulated;the secretion of IL-12 and IFN-？ increased also.The mature BMDCs stimulated the allergic CD4＋T and CD8＋T cells proliferation and their IL-2 and IFN-γ secretion,and the activated CD8＋T cells effectively killed B16-OVA melanoma cells and RMA-S/OVA lymphoma cells in vitro.Conclusion E.coli LLO/OVA is effective in inducing BMDCs maturation via activating TLR4 and NOD1 receptor signalling pathway and promoting specific anti-tumor T cell immunity in vitro.

流产布鲁菌变异株S2308△rfbE感染促进小鼠髓源性树突状细胞(BMDC)成熟和细胞因子释放

目的研究流产布鲁菌变异株S2308△rfbE感染对小鼠髓源性树突状细胞(BMDC)成熟和免疫应答功能的影响。方法采用流式细胞术检测S2308△rfbE感染小鼠BMDC后主要组织相容性抗原复合体Ⅰ(MHCⅠ)、MHCⅡ、CD40、CD86的表达变化,ELISA检测BMDC的肿瘤坏死因子α(TNF-α)、白细胞介素6(IL-6)和IL-10的分泌量。结果S2308△rfbE感染BMDC后,细胞表达MHCⅠ、MHCⅡ、CD40、CD86明显增强,TNF-α、IL-6和IL-10分泌量升高。结论布鲁菌变异株S2308△rfbE促进BMDC成熟和细胞因子分泌。

IL-6抑制LPS诱导的小鼠髓源性DCs成熟的实验研究

目的观察白细胞介素-6(IL-6)对于内毒素(LPS)诱导的小鼠髓源性树突状细胞(DC)成熟效应的抑制作用。方法分离小鼠骨髓细胞,采用黏附法结合GM-CSF和IL-4刺激法在体外培养髓源性DCs(BMDCs)。用相差倒置显微镜观察BM-DCs的形态特点。用LPS诱导DC成熟。采用FACS结合混合淋巴细胞反应,观察IL-6处理与否,LPS诱导的BMDCs在表型和刺激同种淋巴细胞增殖功能上的变化。结果形态观察和FACS分析的结果表明:体外成功培养了纯度较高的高表达CD11c的BMDCs,LPS能明显诱导BMDCs表面MHC-Ⅱ类分子和共刺激分子CD40的表达上调;而经过IL-6处理后,LPS诱导BMDCs表面CD80、CD86、CD40表达上调的能力被显著削弱(P<0.05)。混合淋巴细胞反应显示,与单独用LPS处理的BMDCs相比,经IL-6处理后的BMDCs刺激同种淋巴细胞增殖的能力明显减弱,并呈剂量依赖关系(P<0.05)。结论IL-6能明显抑制LPS诱导的BMDCs成熟,可能是肿瘤免疫逃逸的重要机制之一。

重组疫苗E.coli LLO／OVA经TLR4和NOD1受体诱导树突状细胞表达细胞因子

目的:探讨树突状细胞(DC)的模式识别受体(PPRs)活化与细胞因子表达的关系。方法:采用基因芯片及RT-PCR检测经E.coliLLO/OVA刺激后小鼠骨髓树突状细胞(bone marrow-derived dendritic cell,BMDC)的PPRs及其下游NF-κB信号通路相关分子mRNA的表达水平,并观察BMDC的活化状况及培养上清液内细胞因子含量。结果:经E.coliLLO/OVA刺激后2h,BMDC出现短暂的TLR4mRNA表达上调,其下游信号途径相关的Myd88、Rip2、Irak1、Irak2、Ikkα、NF-κB1和NF-κB2mRNA均出现表达上调,黏附分子Icam1、细胞因子IL-1a、IL-1b、IL-6和TNF-α的mRNA也表达上调;经E.coliLLO/OVA刺激后4h,BMDC出现Card4(NOD1)mRNA表达上调,其下游信号途径相关的Rip2、Ikkβ、NF-κB1和NF-κB2mRNA均出现表达上调,IFN-γ、TNF-β和CD40mRNA也上调表达。经E.coliLLO/OVA刺激后24h,BMDC表达共刺激分子及MHC-II类分子上调;且培养上清液内IL-12和IFN-γ含量增高。结论:重组疫苗E.coliLLO/OVA经TLR4和NOD1受体激活NF-κB信号通路,诱导了小鼠BMDC成熟并表达一系列细胞因子尤其是IL-12和IFN-γ。

猪骨髓源树突状细胞与单核细胞源树突状细胞体外培养和功能鉴别

为比较来源于猪骨髓来源和外周血单核细胞来源的两种树突状细胞的生物学特性,本研究分别从猪骨髓和外周血中分离前体细胞,经重组猪粒细胞集落刺激因子(GM-CSF)和重组猪白细胞介素-4(IL-4)诱导分化为猪骨髓来源树突状细胞(BMDC)和猪单核细胞衍生树突状细胞(MoDC),对这两种来源的树突状细胞进行形态学观察,细胞表型鉴定以及功能检测,并进行比较。结果显示:BMDC和MoDC均具有典型的树突状细胞形态和基本功能;BMDC和MoDC的分子表型为CD172a^(+)MHC II^(+),经LPS刺激后表达升高;BMDC和Mo DC均具有吞噬功能,BMDC吞噬能力较强;在TranswellTM迁移实验中,Mo DC具有更好的迁移能力;BMDC和MoDC均可刺激淋巴细胞增殖,BMDC刺激淋巴细胞增殖率高于MoDC。本研究可为不同体外模型中DCs的选择提供依据。

CD11b激动剂leukadherin-1通过阻断NF-κB p65通路抑制小鼠骨髓来源树突状细胞TLR7和TLR9活化

目的研究整合素CD11b激动剂白细胞黏附素1(LA1)对小鼠骨髓来源的树突状细胞(BMDC)中Toll样受体7(TLR7)和TLR9通路活化的影响,并探索其调控机制。方法成功诱导BMDC,用CCK-8法和异硫氰酸荧光素标记的膜联素Ⅴ/碘化丙啶(annexinⅤ-FITC/PI)双染法筛选出对BMDC活性和凋亡都无影响的LA1浓度。LA1预处理BMDC 2 h后,用TLR7激动剂R837和TLR9激动剂CpG1826刺激BMDC,收集细胞用流式细胞术检测BMDC表面标志CD40、CD86和主要组织相容性复合体Ⅱ(MHC-Ⅱ)的表达;收集细胞培养上清,用ELISA检测白细胞介素6(IL-6)、IL-12p40和肿瘤坏死因子α(TNF-α)的含量;用Western blot法检测BMDC中核因子κB p65(NF-κB p65)的磷酸化水平。结果LA1浓度低于20μmol/L时对BMDC活力和凋亡无影响;LA1预处理显著抑制BMDC中R837和CpG1826诱导的CD40、CD86和MHC-Ⅱ的表达;LA1预处理显著抑制BMDC培养上清中R837和CpG1826诱导的IL-6、IL-12p40和TNF-α的含量;进一步研究发现,LA1预处理显著抑制BMDC中R837和CpG1826激活的NF-κB p65磷酸化水平。结论CD11b激动剂LA1可显著抑制BMDC中TLR7和TLR9通路的活化,且通过NF-κB p65信号通路发挥作用。

DA大鼠骨髓来源的树突状细胞的培养和鉴定

目的分离DA大鼠骨髓来源的树突状细胞(BMDC),并进行体外培养及鉴定。方法取出DA大鼠的股骨、胫骨之间骨髓腔的骨髓细胞,并联合应用重组小鼠粒细胞巨噬细胞集落刺激因子(rmGM-CSF)20 ng/mL和10 ng/mL重组小鼠白细胞介素4(rmIL-4),体外培养7 d,诱导DA大鼠骨髓细胞分化为树突状细胞(DC);ELISA检测未成熟树突状细胞(imDC)培养上清液IL-12水平,倒置显微镜观察BMDC增殖情况以及形态变化,扫描电子显微镜观察DC的形态,流式细胞术分析imDC表面特异性标志物OX62/CD103、CD40、CD80、CD86、主要组织相容性复合体Ⅱ(MHCⅡ)的表达;混合淋巴细胞反应检测imDC诱导T淋巴细胞的增殖能力。结果DA大鼠骨髓细胞经体外培养可获得大量imDC;imDC高表达OX62,低表达CD40、CD80、CD86、MHC-Ⅱ;rmIL-10处理的imDC上清液IL-12含量随着培养时间的延长不断降低,rmIL-4处理组则相反;imDC诱导T淋巴细胞增殖的能力较弱。结论成功建立简易分离培养高纯度的DA大鼠imDC的方法。

树突状细胞来源外泌体通过NF-κB通路影响内皮细胞致促炎因子的变化

目的探讨来源于树突状细胞(DCs)的外泌体对人脐静脉内皮细胞(HUVEC)炎症因子的作用和机制。方法从C57BL/6J小鼠中分离获得骨髓树突状细胞(BMDCs)并培养,采用超速离心法分别从BMDCs及经脂多糖(LPS)诱导成熟的BMDCs培养基中分离获得外泌体、并经电镜扫描及免疫印迹法(WB)验证;构建CD63-GFP慢病毒载体并转染BMDCs细胞,Transwell共培养BMDCs细胞与HUVEC、并用外泌体处理细胞;应用ELISA法检测各组细胞肿瘤坏死因子-α(TNF-α)、白介素-6(IL-6)的浓度,蛋白质印迹法(Western blot)测试p100和p105的磷酸化水平,实时荧光定量聚合酶链式反应(RT-PCR)测试TNF-α和IL-6的mRNA表达水平,利用免疫荧光技术检测HUVEC摄取外泌体的情况。结果激光共聚焦显微镜观察显示,HUVEC能摄取BMDCs来源的外泌体;通过LPS诱导的成熟和未成熟的BMDCs外泌体中的IL和TNF水平无统计学差异;BMDCs与HUVEC共同培养的培养基中IL-6和TNF-α的浓度和p100和p105的磷酸化水平比单纯培养HUVEC培养基中的表达明显升高(P<0.05),但BMDCs外泌体被外泌体抑制剂GW4869抑制后,TNF-α和IL-6含量及p100和p105的磷酸化水平明显下降(P<0.01);共培养联合NF-κB抑制剂BAY11-7082组中的TNF-α和IL-6含量及p100和p105磷酸化水平比单纯HUVEC与BMDCs共培养组明显下降(P<0.001)。结论BMDCs来源的外泌体能够被HUVEC摄取,并促进HUVEC炎症因子TNF-α和IL-6升高,其机制可能与BMDCs来源的外泌体影响NF-κB信号通路中p100以及p105的磷酸化水平有关。

MRP8、MRP14及MRP8/14促进体外培养的小鼠骨髓来源树突状细胞的表型成熟

目的探讨髓样相关蛋白8(MRP8)、MRP14及其异二聚体MRP8/14对小鼠骨髓源性树突状细胞(BMDC)表型成熟的影响。方法体外培养及纯化小鼠BMDC,分为对照组、1μg/m L MRP14处理组、1μg/m L MRP8处理组、1μg/m L MRP8/14处理组。采用流式细胞术检测刺激后BMDC表面共刺激分子CD40、CD80、CD86、主要组织相容性复合体Ⅱ(MHCⅡ)的表达情况。结果 MRP14、MRP8及MRP8/14均能促进BMDC表面共刺激分子CD40、CD80、CD86表达,MRP14、MRP8均能促进BMDC表面共刺激分子MHCⅡ表达,且MRP14和MRP8/14促进BMDC表达CD80、CD86的能力强于MRP8。结论 MRP14、MRP8及MRP8/14通过增加BMDC表面共刺激分子的表达而促进BMDC的表型成熟,且MRP8、MRP14及MRP8/14三者促进DC表达各种共刺激分子的能力不同。