细粒棘球蚴抗原B对小鼠巨噬细胞RAW264.7的极化作用  被引量：1

作　　者：焦红杰 齐文静 郭刚[1] 包建玲[1] 吴川川 宋传龙 李军[1] 张文宝[1,2] 严媚 JIAO Hongjie;QI Wenjing;GUO Gang;BAO Jianling;WU Chuanchuan;SONG Chuanlong;LI Jun;ZHANG Wenbao;YAN Mei(First Affiliated Hospital of Xinjiang Medical University,Urumqi 830054,China;Basic Medical College of Xinjiang Medical University,Urumqi 830054,China)

机构地区：[1]新疆医科大学第一附属医院,乌鲁木齐830054 [2]新疆医科大学基础医学院,乌鲁木齐830054

出　　处：《中国寄生虫学与寄生虫病杂志》2023年第1期23-28,共6页Chinese Journal of Parasitology and Parasitic Diseases

基　　金：国家自然科学基金(82160031,81830066);省部共建中亚高发病成因与防治国家重点实验室立项项目(SKL-HIDCA-2020-BC);新疆维吾尔自治区科技厅天山创新团队项目(2020D14027)。

摘　　要：目的探讨细粒棘球蚴抗原B(AgB)对巨噬细胞极化的调控作用。方法将RAW264.7巨噬细胞培养24 h后,分为M1、M2、AgB、AgB+M1、AgB+M2和空白对照组(M0组),每组3孔。待所有巨噬细胞贴壁3 h后,AgB、AgB+M1、AgB+M2组均加入羊源细粒棘球蚴囊液提取的天然AgB(终浓度为1000 ng/ml),刺激1 h后,M1组和AgB+M1组加入脂多糖(LPS,终浓度为100 ng/ml)和γ干扰素(IFN-γ,终浓度为20 ng/ml)刺激分化20 h;M2组和AgB+M2组加入白细胞介素4(IL-4)、IL-13(终浓度均为20 ng/ml)刺激分化20 h;空白对照组不更换培养液,同步培养20 h。显微镜下观察巨噬细胞形态。提取各组巨噬细胞总RNA,RT-PCR检测刺激后巨噬细胞表面标志物精氨酸酶1(Arg-1)、肿瘤坏死因子α(TNF-α)的mRNA相对转录水平;蛋白质免疫印迹(Western blotting)分析巨噬细胞蛋白Arg-1、诱导型一氧化氮合酶(iNOS)的相对表达量;ELISA检测刺激后巨噬细胞培养上清中IL-10、TNF-α的表达变化。结果经刺激分化后,镜下可见M1组和AgB+M1组巨噬细胞大部分呈不规则形,有触角;M2组和AgB+M2组巨噬细胞大部分呈圆形或椭圆形,极少呈不规则形;M0组和AgB组巨噬细胞部分呈圆形、椭圆形,部分呈不规则形。RT-PCR结果显示,M2组和AgB+M2组巨噬细胞的Arg-1 mRNA相对转录水平分别为189.49±68.43、435.83±123.57(t=246.30,P<0.01),二者均高于M0组(1.00±0.00)、M1组(1.87±1.29)、AgB组(2.37±2.06)、AgB+M1组(3.96±1.92)(t=188.50、187.60、187.10、185.50,均P<0.01;t=434.80、434.00、433.50、431.90,均P<0.01);M1和AgB+M1组巨噬细胞的TNF-αmRNA相对转录水平分别为8.34±2.92、8.10±1.54(t=0.24,P>0.05),二者均高于M0组(1.00±0.00)、M2组(1.37±0.64)、AgB组(2.86±0.44)、AgB+M2组(1.62±0.27)(t=7.34、6.97、5.48、6.71,均P<0.01;t=7.10、6.74、5.24、6.48,均P<0.01)。Western blotting检测结果显示,M2组巨噬细胞的Arg-1蛋白相对表达量为1.18±0.35,高于M1组(0.33±0.18)、AgB+M1组(0.58±0.10)(t=0.67、0.61,均P<0.01)ObjectiveTo investigate the regulatory effect of Echinococcus granulosus antigen B(AgB)on macrophage polarization.MethodsAfter cultivated for 24 h,the RAW264.7 macrophages cells were designated to6 groups:M1,M2,AgB,AgB+M1,AgB+M2 and blank control(M0),3 wells each group.After all the cells attached to the well wall for 3 h,the AgB、AgB+M1、AgB+M2 group was respectively added with natural AgB extracted from sheep hydatid cyst fluid(1000 ng/ml,final concentration);1 h post-stimulation,the M1 and AgB+M1group was respectively added with lipopolysaccharide(LPS,final concentration 100 ng/ml),and IFN-γ(20 ng/ml,final concentration)to stimulate differentiation for 20 h;M2 and AgB+M2 group was added with interleukin 4(IL-4)and IL-13(final concentration 20 ng/ml)to stimulate differentiation for 20 h;the control group was cultured in parallel without changing medium.The morphology of macrophage cells were observed microscopically.Total RNA of the macrophages in all groups was extracted for performing RT-PCR to detect the relative transcription levels of the surface markers on stimulated macrophages,including arginase 1(Arg-1)and tumor necrosis factorα(TNF-α).The relative expression levels of Arg-1 and inducible nitric oxide synthase(iNOS)were analyzed by Western blotting.The change of IL-10 and TNF-αexpression in the culture supernatant of stimulated macrophages were detected by ELISA.ResultsAfter stimulation and differentiation,most cells in the M1 group and AgB+M1 group were irregularly shaped and had antennae.The cells of M2 group and AgB+M2 group were mostly round or oval,and very few were irregular.The cells of M0 group and AgB group were partly round and oval,and partly irregular.RTPCR showed that the relative transcription levels of Arg-1 mRNA in the M2 group and the AgB+M2 group were189.49±68.43 and 435.83±123.57,respectively(t=246.30,P<0.01).They were higher than those in the M0group(1.00±0.00),M1 group(1.87±1.29),AgB group(2.37±2.06),AgB+M1 group(3.96±1.92)(t=188.50,187.60,187.10,185.50,P<0.01;t=434.80,

关 键 词：细粒棘球绦虫 分泌抗原 抗原B 巨噬细胞极化 

分 类 号：R383.33[医药卫生—医学寄生虫学]