TNFR2基因的CA重复多态性在两个独立的白人群体中与肥胖表型的连锁和关联(英文)

我们先前通过全基因组扫描发现1p36与体重指数显提示性连锁(LOD=2.09)。肿瘤坏死因子受体2(TNFR2)定位于1p36,是肥胖的一个极好的图位和功能侯选基因。本研究采用数量传递连锁不平衡检验在两个大的独立的白人样本中进行了TNFR2基因与肥胖表型的连锁与关联检验。第一组受试者由来自79个多代家系的1836个个体组成;第二组受试者由来自157个核心家庭的636个个体组成。所检测的肥胖表型包括体重指数、脂肪量和脂肪量百分数。在多代家系中我们发现TNFR2基因变异与BMI显著连锁(P=0.0056)。结果表明,TNFR2基因是影响白人BMI变异的一个数量性状位点。

CD4^+ TNFR2^+ 调节性T细胞在免疫相关疾病中作用机制的研究进展

调节性T细胞(Treg)是一种具有免疫抑制功能的效应性T淋巴细胞,在维持机体的免疫自稳中发挥重要作用。肿瘤坏死因子受体2(TNFR2)主要表达于淋巴细胞并参与调节淋巴细胞的分化和存活。TNFR2可以稳定CD4^+CD25^+Treg的数量及其抑制功能。作为人和小鼠体内抑制功能最强的Treg,CD4和肿瘤坏死因子受体双阳性(CD4^+TNFR2^+)Treg参与多种疾病如肿瘤、移植排斥、结肠炎、关节炎、寄生虫感染等的免疫反应过程。CD4^+TNFR2^+Treg在各种免疫相关疾病中的作用及其机制已成为新的研究热点。

TNFR2与三氯乙烯致敏小鼠免疫性肝损伤的关系研究

目的观察三氯乙烯(TCE)致敏小鼠肝脏内TNFR2表达情况,探讨TNFR2与免疫性肝脏损伤之间的关系。方法选取21只SPF级雌性BALB/c小鼠,6~8周龄,随机将其分为空白对照组(5只),溶剂对照组(5只),TCE处理组(11只),建立TCE致敏小鼠模型,进行小鼠背部皮肤致敏反应评分,评分大于1分为TCE致敏组,反之为未致敏组。模型完成后处死小鼠,摘取眼球取血,测定血清肝功能活性指标ALT和AST;取出小鼠肝脏制成石蜡切片,HE染色观察小鼠肝脏病理表现,免疫组织化学(IHC)法和Western blot法观察小鼠肝脏肿瘤坏死因子(TNF)-α与TNFR2的表达情况。实时荧光定量PCR法检测TNFR2的mRNA水平。结果TCE组致敏率为45.45%(5/11);致敏组小鼠的肝功能指标较高,与其他组比较差异有统计学意义(P<0.05)。HE染色结果显示TCE致敏组可见细胞发生空泡样变性,细胞呈蜂窝状且胞质疏松,其余组小鼠的肝细胞形态正常,染色均匀。免疫组化实验显示,TCE致敏组TNF-α表达较高,且与其他组相比TCE致敏组可以观察到大量TNFR2阳性表达,评分结果差异有统计学意义(P<0.05)。实时荧光PCR结果显示TCE致敏组TNFR2的mRNA表达也比其他组表达升高(P<0.05)。Western blot实验表明TCE致敏组比其他组TNFR2蛋白表达水平增高,差异有统计学意义(P<0.05)。结论TNFR2在TCE致敏组小鼠肝脏中表达升高,其表达的改变可能参与了TCE致敏小鼠免疫性肝脏损伤过程。

Up-regulation of tumor necrosis factor-a pathway survival genes and of the receptor TNFR2 in gastric cancer

BACKGROUND Gastric carcinogenesis can be induced by chronic inflammation triggered by Helicobacter pylori(H. pylori) infection. Tumor necrosis factor(TNF)-α and its receptors(TNFR1 and TNFR2) regulate important cellular processes, such as apoptosis and cell survival, and the disruption of which can lead to cancer. This signaling pathway is also modulated by microRNAs(miRNAs), altering gene expression.AIM To evaluate the mRNA and miRNAs expression involved in the TNF-α signaling pathway in gastric cancer(GC) tissues and its relationship.METHODS Quantitative polymerase chain reaction(qPCR) by TaqMan? assay was used to quantify the RNA transcript levels of TNF-α signaling pathway(TNF, TNFR1,TNFR2, TRADD, TRAF2, CFLIP, NFKB1, NFKB2, CASP8, CASP3) and miRNAs that targets genes from this pathway(miR-19 a, miR-34 a, miR-103 a, miR-130 a,miR-181 c) in 30 GC fresh tissue samples. Molecular diagnosis of H. pylori was performed by nested PCR for gene HSP60. A miRNA:mRNA interaction network was construct using Cytoscape v3.1.1 from the in silico analysis performed using public databases.RESULTS Up-regulation of cellular survival genes as TNF, TNFR2, TRADD, TRAF2, CFLIP,and NFKB2, besides CASP8 and miR-34 a was observed in GC tissues, whereas mediators of apoptosis such as TNFR1 and CASP3 were down-regulated. When the samples were stratified by histological type, the expression of miR-103 a and miR-130 a was significantly increased in the diffuse-type of GC compared to the intestinal-type. However, no influence of H. pylori infection was observed on the expression levels of mRNA and miRNAs analyzed. Moreover, the miRNA:mRNA interaction network showed several interrelations between the miRNAs and their target genes, highlighting miR-19 a and miR-103 a, which has as predicted or validated target a large number of genes in the TNF-α pathway,including TNF, TNFR1, TNFR2, CFLIP, TRADD, CASP3 and CASP8.CONCLUSION Our findings show that cell survival genes mediated by TNF/TNFR2 binding is up-regulated in GC favoring its pro-tumoral effect, while pro-apoptotic genes as CASP3 and TNFR1 are down-regulated, indicating disbalance between apoptosis and cell proliferation processes in this neoplasm. This process can also be influenced by an intricate regulatory network of miRNA:mRNA.

Downregulation of TNFR2 decreases survival gene expression,promotes apoptosis and affects the cell cycle of gastric cancer cells

BACKGROUND Chronic inflammation due to Helicobacter pylori(H.pylori)infection promotes gastric carcinogenesis.Tumour necrosis factor-α(TNF-α),a key mediator of inflammation,induces cell survival or apoptosis by binding to two receptors(TNFR1 and TNFR2).TNFR1 can induce both survival and apoptosis,while TNFR2 results only in cell survival.The dysregulation of these processes may contribute to carcinogenesis.AIM To evaluate the effects of TNFR1 and TNFR2 downregulation in AGS cells treated with H.pylori extract on the TNF-αpathway.METHODS AGS cell lines containing TNFR1 and TNFR2 receptors downregulated by specific shRNAs and nonsilenced AGS cells were treated with H.pylori extract for 6 h.Subsequently,quantitative polymerase chain reaction with TaqMan®assays was used for the relative quantification of the mRNAs(TNFA,TNFR1,TNFR2,TRADD,TRAF2,CFLIP,NFKB1,NFKB2,CASP8,CASP3)and miRNAs(miR-19a,miR-34a,miR-103a,miR-130a,miR-181c)related to the TNF-αsignalling pathway.Flow cytometry was employed for cell cycle analysis and apoptosis assays.RESULTS In nonsilenced AGS cells,H.pylori extract treatment increased the expression of genes involved in cell survival and inhibited both apoptosis(NFKB1,NFKB2 and CFLIP)and the TNFR1 receptor.TNFR1 downregulation significantly decreased the expression of the TRADD and CFLIP genes,although no change was observed in the cellular process or miRNA expression.In contrast,TNFR2 downregulation decreased the expression of the TRADD and TRAF2 genes,which are both important downstream mediators of the TNFR1-mediated pathway,as well as that of the NFKB1 and CFLIP genes,while upregulating the expression of miR-19a and miR-34a.Consequently,a reduction in the number of cells in the G0/G1 phase and an increase in the number of cells in the S phase were observed,as well as the promotion of early apoptosis.CONCLUSION Our findings mainly highlight the important role of TNFR2 in the TNF-αpathway in gastric cancer,indicating that silencing it can reduce the expression of survival and anti-apoptotic genes.

斑马鱼TNFR2基因克隆及表达分析

利用巢式PCR方法克隆斑马鱼(Danio rerio)肿瘤坏死因子受体2(TNFR2)基因,该基因全长1 242bp,编码413个氨基酸,分子质量44.68 ku,等电点5.90。实时荧光定量PCR结果表明,TNFR2基因在斑马鱼胚胎发育时期的表达量呈现下降后趋于稳定,在斑马鱼不同组织中均能检测到,并且表达丰度差别不大,在肌肉中表达量最高,在肠道中表达量最低。

The TNFα/TNFR2 axis mediates natural killer cell proliferation by promoting aerobic glycolysis

Natural killer(NK)cells are predominant innate lymphocytes that initiate the early immune response during infection.NK cells undergo a metabolic switch to fuel augmented proliferation and activation following infection.Tumor necrosis factor-alpha(TNFα)is a well-known inflammatory cytokine that enhances NK cell function;however,the mechanism underlying NK cell proliferation in response to TNFαis not well established.Here,we demonstrated that upon infection/inflammation,NK cells upregulate the expression of TNF receptor 2(TNFR2),which is associated with increased proliferation,metabolic activity,and effector function.Notably,IL-18 can induce TNFR2 expression in NK cells,augmenting their sensitivity toward TNFα.Mechanistically,TNFα-TNFR2 signaling upregulates the expression of CD25(IL-2Rα)and nutrient transporters in NK cells,leading to a metabolic switch toward aerobic glycolysis.Transcriptomic analysis revealed significantly reduced expression levels of genes involved in cellular metabolism and proliferation in NK cells from TNFR2 KO mice.Accordingly,our data affirmed that genetic ablation of TNFR2 curtails CD25 upregulation and TNFα-induced glycolysis,leading to impaired NK cell proliferation and antiviral function during MCMV infection in vivo.Collectively,our results delineate the crucial role of the TNFα-TNFR2 axis in NK cell proliferation,glycolysis,and effector function.

重组融合蛋白TNFR2-Fc-IL-1ra抑制血管紧张素Ⅱ诱导的小鼠心肌肥厚

目的探讨新型重组融合蛋白TNFR2-Fc-IL-1ra(TFI)对高血压心肌肥厚的抑制作用及可能机制。方法8周龄雄性C57BL/6J健康小鼠24只随机分为3组:对照组(生理盐水)、模型组[血管紧张素Ⅱ(AngⅡ)1500ng/(kg·min),灌注7d]、治疗组[AngⅡ1500ng/(kg·min)+TFI 5mg/(kg·2d)],每组8只。第7天时采用鼠尾套法检测尾动脉血压、超声检测心脏结构及功能;即刻处死并取其心脏进行组织切片,行苏木素-伊红(HE)染色观察大体形态;麦胚凝集素(WGA)染色观察心肌细胞肥大;免疫组化染色检测各组心肌中肿瘤坏死因子α(TNF-α)、白细胞介素1β(IL-1β);实时定量PCR检测TNF-α、IL-1β和心房钠尿肽(ANP)、β-肌球蛋白重链(β-MHC)的mRNA水平。结果与对照组相比,模型组1、3、7d的血压明显升高;左心室舒张、收缩末期前壁厚度增厚;心肌细胞横截面面积[(322.2±11.6)比(199.7±12.4)μm2]明显升高;TNF-α[(1.33±0.26)%比(0.03±0.01)%]和IL-1β[(1.84±0.33)%比(0.08±0.03)%]阳性面积增加;TNF-α、IL-1β、ANP和β-MHC mRNA表达升高(均P<0.05)。与模型组相比,治疗组小鼠血压无明显变化;心室壁厚度减轻;心肌细胞横截面面积减小;TNF-α、IL-1β表达降低;ANP和β-MHC mRNA表达降低(均P<0.05)。结论 TFI通过抑制炎症反应改善心肌肥厚。

Myeloid-derived suppressor cells promote B-cell production of IgA in a TNFR2-dependent manner

Myeloid-derived suppressor cells(MDSCs)are well known for their capacity to suppress antitumor T-cell responses,but their effects on B-cell function and antibody production remain unclear.Here,we found that MDSCs that accumulated around the germinal center in the spleen of tumor-bearing mice co-located with B cells.In the presence of MDSCs,the antibody reaction to a surrogate antigen was significantly enhanced in mice,especially the immunoglobulin(Ig)A subtype.Co-culture with MDSCs promoted both proliferation and differentiation of B cells into IgA-producing plasma cells in vitro.Interestingly,the cross talk between MDSCs and B cells required cell-cell contact.MDSCs from tumor necrosis factor receptor(TNFR)2^(−/−)mice,but not from TNFR1^(−/−)mice,failed to promote B-cell responses.Further investigation suggested that interleukin-10 and transforming growth factor-β1 were crucial for the MDSC-mediated promotion of IgA responses.These results demonstrate a novel mechanism of MDSC-mediated immune regulation during tumor growth.

肿瘤坏死因子受体及其信号转导蛋白TRAF2在喉癌中的表达

目的:探讨肿瘤坏死因子受体(TNFR)和其转导蛋白TRAF2的表达及其与喉鳞状细胞癌生物学行为的关系。方法:利用免疫组织化学及原位末端标记法,对33例喉鳞状细胞癌组织TNFR1、TNFR2和TRAF2的表达及其凋亡指数进行检测。结果:①33例喉鳞状细胞癌中,21例TNFR1表达阳性(63.6%),2例TNFR2表达阳性(6.1%),两者表达染色阳性部位主要集中在细胞膜上,表达程度与喉鳞癌的生物学行为无关(P>0.05);②33例喉鳞状细胞癌中,23例TRAF2表达阳性(69.7%),其表达部位主要位于细胞浆中。TRAF2的表达程度与喉鳞癌的病理分级有关(P<0.05),与其他的生物学行为无关(P>0.05);③TRAF2的表达与TNFR1的表达具有明显的正相关(r=0.637,P<0.01);④TNFR1、TRAF2表达阳性组织的细胞凋亡指数(3.12±1.47及2.85±1.19)显著低于TNFR1、TRAF2表达阴性组织(4.28±1.34及5.12±0.81)(P<0.05及P<0.01)。结论:TNFR1信号转导过程中募集TRAF2增强肿瘤细胞抗凋亡能力,与肿瘤的分化和恶性程度有一定关系,缺乏表达TNFR2可能对喉癌的发生发展有一定作用。

肿瘤坏死因子受体2突变载体对巨噬细胞炎症反应的影响

目的探讨肿瘤坏死因子受体超家族1B(TNFRSF1B)196位基因多态性(T突变为G)与巨噬细胞TNF/TNFR2信号通路介导炎症反应的相关性。方法运用基因重组技术构建真核表达载体pcDNA6.0-TNFR2196Met和pcDNA6.0-TNFR2196Arg,采用脂质体转染法分别转染至巨噬细胞中,转染48 h后使用杀稻瘟菌素抗性筛选4周,建立稳定转染细胞系。将酶消化法培养的巨噬细胞分为四组:空白对照组、pcDNA6.0空质粒组、pcDNA6.0-TNFR2196Met组及pcDNA6.0-TNFR2196Arg组。采用酶切及测序法鉴定重组质粒,RT-PCR检测肿瘤坏死因子受体2(TNFR2)、cIAP1、cIAP2mRNA的变化;Western blot检测p-JNK、cIAP1、cIAP2、TNFR2及核因子κB(NF-κB)的蛋白表达;ELISA检测细胞上清液可溶性TNFR2(sTNFR2)、白细胞介素1β(IL-1β)和白细胞介素6(IL-6)水平。结果酶切测序结果显示成功构建了TNFR2基因196Met和196Arg表达载体。转染到巨噬细胞后,与空白对照组和pcDNA6.0空质粒组比较,pcDNA6.0-TNFR2196Arg组、pcDNA6.0-TNFR2196Met组TNFR2、cIAP1、cIAP2、IL-1β、IL-6和p-JNK的表达增高(P<0.05);与pcDNA6.0-TNFR2196Met组比较,pcDNA6.0-TNFR2196Arg组TNFR2、cIAP1、cIAP2、IL-1β、IL-6和pJNK的表达明显降低(P<0.05),TNFR2196Arg介导的NF-κB活性显著降低。结论成功构建稳定表达TNFR2196Met、TNFR2196Arg载体,TNFR2突变通过TNF/TNFR2信号通路介导炎症反应,可能是参与慢性炎症性疾病的作用机制。

TNFα诱导血管内皮细胞HO-1基因表达的受体及细胞内信号机制

目的探讨肿瘤坏死因子(TNFα)对脑微血管内皮细胞(BMVEC)HO-1基因表达的信号转导机制。方法采用TNF受体1敲除的脑血管内皮细胞[BVEC/TNF-RI(-/-)]为研究对象,用RT-PCR法测定TNFα刺激细胞24h后HO-1基因mRNA的表达,用westernblot法检测TNFα对JNK、ERK激酶和转录因子AP-1活性的影响,并用JNK或ERK抑制剂干预上述诱导实验。结果TNFα刺激BVEC/TNF-RI(-/-)HO-1表达增高(P<0.05),此外,TNFα刺激BVEC/TNF-RI(-/-)可引起JNK和ERK激酶表达和转录因子AP-1的活性增强(P<0.05),可是JNK的抑制剂SP600125能减弱TNF诱导的HO-1的表达(P<0.05),而ERK的抑制剂不能。结论TNFR2和JNK激酶对于TNFα诱导的HO-1的表达有重要作用。

肿瘤坏死因子受体1和2在胎膜早破胎膜组织中的表达及作用

目的探讨肿瘤坏死因子受体1和受体2在胎膜早破发病机制中的作用。方法足月前胎膜早破(早产组)、足月胎膜早破(胎膜早破组)和足月妊娠择期剖宫产(剖宫产组)产妇各8例,采用WesternBlot-ting方法检测其胎膜组织中TNFR1和TNFR2的蛋白表达。结果(1)TNFR1表达:胎膜早破组为(0.2102±0.0157),早产组为(0.2071±0.0178),剖宫产组为(0.1182±0.0058),胎膜早破组和早产组TNFR1表达水平高于剖宫产组,差异有显著性(P<0.05),而胎膜早破组与早产组比较差异无显著性(P>0.05);TNFR2表达:剖宫产组为(0.2121±0.0148),早产组为(0.1339±0.0324),胎膜早破组为(0.1164±0.0386),剖宫产组TNFR2表达水平高于胎膜早破组和早产组,差异有显著性(P<0.05),而胎膜早破组和早产组比较差异无显著性(P>0.05)。结论胎膜上可能存在TNFR的某种转化途径,胎膜早破的发生可能是由于局部TNF-α水平升高诱导胎膜上TNFR由TNFR2向TNFR1转化,启动胎膜细胞凋亡,从而导致胎膜的破裂。

Cyclophosphamide abrogates the expansion of CD4^(+)Foxp3^(+) regulatory T cells and enhances the efficacy of bleomycin in the treatment of mouse B16-F10 melanomas

Objective:Promotion of the proliferative expansion of CD4^(+)Foxp3^(+)regulatory T cells(Tregs)is one of the side effects that limits the use of bleomycin(BLM)in the treatment of tumors.In this study,we examined the hypothesis that cyclophosphamide(CY),a chemotherapeutic agent with the capacity to eliminate tumor infiltrating Tregs,abrogated BLM-induced expansion of Tregs and consequently resulted in a better anti-tumor effect.Methods:The in vitro effects of BLM,with or without mafosfamide(MAF,the active metabolite of CY),on both TGF-β-induced differentiation of Tregs(iTregs),and TNF-induced expansion of naturally occurring Tregs(nTregs)were assessed.The in vivo effect of low doses of BLM and CY on tumor-infiltrating Tregs,as well as on the growth of mouse B16-F10 melanomas,was also studied.Results:In vitro treatment with BLM promoted the differentiation of iTregs,as well as TNF-induced expansion of nTregs.These effects of BLM were completely abrogated by MAF.Furthermore,in the mouse B16-F10 melanoma model,treatment with low doses of BLM increased the number of tumor-infiltrating Tregs,and this effect of BLM was also abrogated by CY.Importantly,combination therapy with low doses of BLM and CY showed synergistic anti-tumor effects.Conclusions:CY abrogated the effect of BLM on the expansion of Tregs.The combination of these 2 chemotherapeutic agents may represent a safer and more effective therapy in the treatment of cancer patients,and thus merits future clinical evaluation.

大鼠膝关节给药rAAV2/TNFR:Fc毒性研究

目的给大鼠膝关节腔注射rAAV2/TNFR:Fc,观察供试品对机体产生的毒性反应及其严重程度、主要毒性靶器官及损害的可逆程度。方法设PBS对照组、人源低剂量组、人源中剂量组、人源高剂量组、鼠源低剂量组、鼠源高剂量组、PBS对照卫星组、人源低剂量卫星组和人源高剂量卫星组,共9个组,分别给予PBS、人源1×1012vg/ml、2×1012vg/ml、3×1012vg/ml、鼠源1×1012vg/ml、3×1012vg/ml、PBS、人源1×1012vg/ml及人源3×1012vg/ml的药物。试验采用膝关节腔注射,每次注射50μl,连续给药8d,每次注射单侧膝关节,左右侧膝关节交替注射,末次给药后连续观察3个月。结果动物的临床症状、尿生化、体温、血液学、血清生化学、脏器重量等均未见生物学意义的改变,病理学检查也未发现与供试品相关的组织病理学改变。关节腔注射后的主要分布组织为:关节腔滑膜、脾脏和淋巴结,随时间延长,供试品在各组织脏器的分布浓度有下降的趋势。大鼠膝关节腔注射给药rAAV2/hTNFR:Fc,动物体内会产生抗AA2结合抗体、抗hTNFR抗体和中和抗体。结论给大鼠关节腔注射rAAV2/TNFR:Fc,连续给药8d的无明显毒副反应剂量为1.5×1011vg/只。

TNFR 2 M196R Polymorphism and Acne Vulgaris in Han Chinese:A Case-control Study

In this case-control study,the relationship between M196R(676 T→G) variant in exon 6 of tumor necrosis factor receptor type 2(TNFR2) gene and genetic susceptibility of acne vulgaris in Han Chinese was investigated.A total of 93 acne vulgaris patients and 90 healthy subjects from Han Chinese ethnic group were enrolled in this study.Polymerase chain reaction-restriction fragment length polymorphism(PCR-RFLP) technique was adopted to analyze the single nucleotide polymorphisms(SNPs) of TNFR2 M196R gene,and to examine the association between acne vulgaris and the polymorphisms in TNFR2 M196R gene.The relationship between different genotypes and the susceptibility of acne vulgaris was analyzed.The results showed that there was significant difference in the frequency of the genotype M/R+R/R in the TNFR2 M196R genetic polymorphisms between acne vulgaris patients and healthy controls(χ2=4.343;P=0.037;OR=1.899;95% CI:1.036-3.445);and there was significant difference in the allele(R) frequency between acne vulgaris patients and healthy controls(χ2=5.588;P=0.018;OR=1.838;95% CI:1.105-3.057).It was concluded that the high frequency of 196R allele in the functional M196R polymorphism of TNFR2 is a risk factor for acne vulgaris in Han Chinese.

RECS1负调控肿瘤坏死因子受体2介导的NF-κB激活

RECS1(responsive to centrifugal force and shear stress gene 1)是一血液剪切力应答蛋白.RECS1基因敲除的小鼠年老时易患主动脉囊性中层坏死并表现有大动脉扩张症,暗示RECS1可能参与调控血管的发育重塑.免疫组化分析发现,RECS1基因敲除(RECS1 knockout,RECS1 KO)的小鼠主动脉基质金属蛋白酶-9(matrix metalloproteinase-9,MMP-9)的表达水平明显提高,但RECS1的结构与功能及相关作用机理仍不清楚.研究发现,RECS1是肿瘤坏死因子受体2(tumor neucrosisfactor receptor 2,TNFR2)的结合蛋白质.报告基因检测实验表明,RECS1能特异地抑制TNFR2特异的激动性抗体或过量表达TNFR2诱导的核转录因子-κB(nuclear factor-κB,NF-κB)活化.NPLY模体缺失突变的RECS1不能结合TNFR2,并丧失对TNFR2介导NF-κB活化的抑制能力.稳定表达RECS1的MEFS细胞中,TNFR2特异的激动性抗体诱导的IκB(inhibitor of NF-κB)降解和NF-κB靶基因白介素-6(interleukin-6,IL-6)的表达均受到明显抑制.该研究揭示了RECS1通过与TNFR2的相互作用,负调控TNFR2介导肿瘤坏死因子信号传递的新功能及RECS1参与血管发育重塑调控的可能机制.

益气血法调节GDF9、c-IAP1/2、JNK1/2、TNFR1/2表达对超排卵大鼠卵巢颗粒细胞凋亡的影响

目的观察益气血法经后增殖方含药血清基于p38 MAPK/核转录因子-κB(NF-κB)信号通路调节生长分化因子9(GDF9)、细胞凋亡抑制蛋白1/2(c-IAP1/2)、c-Jun氨基末端激酶1/2(JNK1/2)、肿瘤坏死因子受体1/2(TNFR1/2)表达对控制性超排卵大鼠卵巢颗粒细胞凋亡的影响。方法取12只雌性大鼠,随机分为控制性超排卵+中药组(6只大鼠给予经后增殖方4.5 g/kg灌胃)和控制性超排卵组(6只大鼠给予等体积生理盐水灌胃),后续经腹腔注射醋酸曲普瑞林、孕马血清促性腺激素、HCG后,取2组大鼠腹主动脉血制备含药血清和空白血清。另取15只雌性大鼠,经腹腔注射醋酸曲普瑞林、孕马血清促性腺激素、HCG后,收集卵巢颗粒细胞,分别与空白血清(空白血清组)、含药血清(含药血清组)、含药血清+GDF9抗体(含药血清+GDF9抗体组)在体外共同培养。TUNEL检测卵巢颗粒细胞凋亡率,qRT-PCR法检测卵巢颗粒细胞中p38 MAPK、NF-κB、GDF9、c-IAP1、c-IAP2、JNK1、JNK2、TNFR1、TNFR2 mRNA表达情况,Western blot法检测卵巢颗粒细胞中GDF9蛋白表达情况。结果含药血清组和含药血清+GDF9抗体组细胞凋亡率均明显低于空白血清组(P均<0.05),且含药血清组明显低于含药血清+GDF9抗体组(P<0.05)。含药血清组p38 MAPK、NF-κB mRNA相对表达量均明显低于空白血清组(P均<0.05)。含药血清组和含药血清+GDF9抗体组c-IAP1、c-IAP2、GDF9 mRNA相对表达量和GDF9蛋白相对表达量均明显高于空白血清组(P均<0.05),且含药血清组均明显高于含药血清+GDF9抗体组(P均<0.05);含药血清组和含药血清+GDF9抗体组JNK1、JNK2、TNFR1、TNFR2 mRNA相对表达量均明显低于空白血清组(P均<0.05),且含药血清组均明显低于含药血清+GDF9抗体组(P均<0.05)。结论益气血法经后增殖方可通过调控p38 MAPK/NF-κB信号通路,上调控制性超排卵大鼠卵巢颗粒细胞中GDF9、c-IAP1、c-IAP2的表达,下调JNK1、JNK2、TNFR1、TNFR2的表达,抑制卵巢颗粒细胞凋亡。

Stimulation of TNF receptor type 2 expands regulatory T cells and ameliorates established collagen-induced arthritis in mice

Tumor necrosis factor(TNF)and its receptors TNF receptor type 1(TNFR1)and type 2(TNFR2)have a central role in chronic inflammatory diseases.While TNFR1 mainly confers inflammation,activation of TNFR2 elicits not only pro-inflammatory but also anti-inflammatory effects.In this study,we wanted to investigate the anti-inflammatory therapeutic potential of selective activation of TNFR2 in mice with established collageninduced arthritis.Mice with established arthritis induced by immunization with bovine collagen type II were treated with six injections of the TNFR2-specific agonist TNCscTNF80,given every second day.Two days after treatment cessation,the cell compositions of bone marrow,spleen and lymph nodes were analyzed.Mice were visually scored until day 30 after the start of therapy and the degree of joint inflammation was determined by histology.Treatment with TNCscTNF80 increased arthritis-induced myelopoiesis.Little effect was seen on the infiltration rate of inflammatory immature myeloid cells and on the reduction of lymphoid cells in secondary lymphoid organs.Upon treatment,frequency of regulatory T(Treg)cells in the CD4+T-cell population was increased in both spleen and inguinal lymph nodes.In addition,the expression of TNFR2 on Treg cells was enhanced.The clinical score started to improve 1 week after cessation treatment and remained lower 30 days after initiation of therapy.The histological score also revealed amelioration of joint inflammation in TNCscTNF80-treated versus control mice.Activation of TNFR2 might provide a suitable therapeutic strategy in autoimmune arthritis by increasing the numbers of regulatory cell types,in particular Treg cells,and by attenuation of arthritis.

肿瘤坏死因子样配体1A与炎症发生发展的关系

肿瘤坏死因子样配体1A(TNF-like ligand 1 aberrance,TL1A)作为新近发现的TNF家族成员,通过与其受体—死亡受体3(DR3)和诱骗受体(DcR3/TR6)结合,抑制内皮细胞的生长,是天然存在的血管内环境稳态的调节者。TL1A与IL-12和IL-23分别协同刺激Th1和Th17,参与免疫应答,尤其是在炎症中表达或表达增加,诱导多种致炎因子IFN-γ、IL-8、IL-13、TNF-α、MPC-1以及黏附分子ICAM-1、VCAM-1等表达增多,在炎性疾病的发生、发展中起重要作用。