MBD2 promotes Th2 differentiation in ovalbumin-induced CD4+T cells

Introduction:Allergen-specific CD4+T cells play a central role in autoimmune disorders,allergies and asthma,with Th2-type immunity being the typical functional response of CD4+T cells.This study aimed to investigate the role of MBD2 in regulating Th2 cell differentiation.Methods:Splenic mononuclear cells were extracted from C57BL/6 mice,and CD4+T cells were isolated using magnetic beads and confirmed through flow cytometry.Lentivirus was employed to construct MBD2-silenced CD4+T cells.In vitro experiments were performed to treat splenogenic mononuclear cells and CD4+T cells with Ovalbumin(OVA),and Th2 cell ratios and IL-4 levels were assessed using flow cytometry and ELISA.Results:The purity of the isolated CD4+T cells was 95.73%,confirming successful isolation of primary CD4+T cells.Compared to the control group,the Th2 cell ratio exhibited an increase in the Th2-induced group.Treatment with 5-Aza(concentrations,1-100μM)promoted Th2 cell differentiation and increased IL-4 levels.Notably,when combined with Th2 induction and 10μM 5-Aza treatment,silencing MBD2 further amplified Th2 cell ratios and elevated IL-4 levels in cell supernatants.Furthermore,OVA(concentration,200μg/mL)induced the differentiation of CD4+T cells into Th2 cells and increased IL-4 secretion.Interestingly,silencing MBD2 significantly increased the Th2 cell ratio and IL-4 levels in OVA-treated CD4+T cells.Conclusion:In summary,OVA promoted CD4+T cell differentiation into Th2 cells and enhanced IL-4 levels.MBD2 was identified as a mediator of Th2 cell differentiation in splenic-derived CD4+T cells,influenced by OVA or 5-Aza treatment.

GATA-3 promotes Th2 responses through three different mechanisms： induction of Th2 cytokine production, selective growth of Th2 cells and inhibition of Thl cell-specific factors

Naive CD4 T cells can differentiate into at least two different types ofT helpers, Thl and Th2 cells. Th2 cells, capable of producing IL-4, IL-5 and IL-13, are involved in humoral immunity against extracellular pathogens and in the induction of asthma and other allergic diseases. In this review, we summarize recent reports regarding the transcription factors involved in Th2 differentiation and cell expansion, including StatS, Gfi- 1 and GATA-3. Stats activation is necessary and sufficient for IL-2-mediated function in Th2 differentiation. Enhanced Stats signaling induces Th2 differentiation independent of IL-4 signaling; although it does not up-regulate GATA-3 expression, it does require the presence of GATA-3 for its action. Gfi-1, induced by IL-4, promotes the expansion of GATA-3-expressing cells. Analysis of conditional Gata3 knockout mice confirmed the critical role of GATA-3 in Th2 cell differentiation （both IL-4 dependent and IL-4 independent） and in Th2 cell proliferation and also showed the importance of basal GATA-3 expression in inhibiting Thl differentiation.

骨髓间充质干细胞对肺纤维化大鼠肺组织中Thl／Th2平衡的调节作用

目的：观察博莱霉素诱导的肺纤维化大鼠肺组织中Thl型细胞因子干扰素У（IFN-У）和Th2细胞因子白介素4（IL-4）的动态变化，并探讨骨髓问充质干细胞（BMSCs）对Thl／Th2平衡的调节作用。方法：健康雌性SD大鼠随机分为对照组、模型组、BMSCs组。采用气管内注射博莱霉素法（5mg／kg）制作大鼠肺纤维化模型，并给予BMSCs干预治疗。分别于造模后7、14d取肺组织。采用H-E染色法观察肺组织形态学改变；羟脯氨酸检测定量分析肺组织中总胶原蛋白的含量；免疫组织化学检测IFN-У、IL-4在肺组织中的分布及定位；免疫印迹检测IFN-У、IL-4的蛋白表达量。结果：与正常组大鼠相比，模型组大鼠肺组织有较多炎细胞浸润，纤维组织增生及胶原沉积；羟脯氨酸含量显著增加；IFN-У蛋白表达明显下调，IL-4的蛋白表达明显上调。与模型组大鼠相比，BMSCs组大鼠肺组织病理改变显著减轻；羟脯氨酸含量明显减少；IFN-У表达显著上调，但仍低于正常组表达水平；IL-4的表达显著下调，但仍高于正常组表达水平。结论：博莱霉素诱导的肺纤维化大鼠模型中存在Thl／Th2失衡现象，BMSCs移植可减缓其纤维化程度及病理进程，通过对Thl／Th2的调节作用实现。

T-bet与Thl/Th2在乙型肝炎中的作用机制

T-bet是T-box家族的一种重要转录因子,在CD4+T细胞Thl型的分化中起重要作用,并抑制Th2细胞因子合成,可使完全分化的Th2逆转为Th1。目前已证实多种疾病的发生、发展和预后涉及Thl/Th2分化失衡。而T-bet对Thl/Th2分化调控作用在疾病中的作用机制有助于解释疾病的发展机制,为疾病的治疗提供依据。文中就T-bet在乙型肝炎中的作用机制作一综述。

血塞通注射液联合阿司匹林治疗老年缺血性卒中疗效及对患者血清Thl/Th2细胞因子水平的影响

目的:探讨血塞通注射液联合阿司匹林治疗老年缺血性卒中的疗效及对血清Thl/Th2细胞因子水平的影响。方法:选择老年缺血性卒中患者300例,随机分为对照组和观察组各150例。所有患者均进行改善脑循环及相应合并症对症治疗,对照组给予阿司匹林肠溶片治疗,观察组在对照组基础上给予血塞通注射液治疗,比较两组治疗前后FMA、MBI评分、NIHSS评分、IFN-γ、IL-4因子变化及临床疗效和生活质量水平情况。结果:治疗后,观察组中医证候积分比对照组下降更明显(P<0.05);治疗后,两组IL-6及IL-4水平均降低,IFN-γ及IL-2均升高;观察组IL-6及IL-4水平低于对照组,IL-2及IFN-γ高于对照组(P<0.05);两组患者治疗后FMA、MBI评分明显升高,而NIHSS评分明显降低,观察组改善更明显(P<0.05)。治疗后两组NSE、BNP水平明显下降,NGF水平明显上升,观察组更明显(P<0.05)。观察组基本治愈率46.67%,总有效率95.33%均高于对照组24.67%及88.00%(P<0.05)。观察组治疗后QLQ-C30评分显著高于对照组(P<0.05)。结论:血塞通注射液联合阿司匹林可显著改善老年缺血性卒中患者脑神经功能缺损状况,调节机体Thl/Th2细胞因子水平,疗效显著。

联合免疫治疗对复发性自然流产患者外周血Thl/Th2的影响

目的观察联合淋巴细胞免疫、免疫球蛋白和阿司匹林的疗法对复发性自然流产(RSA)患者外周血Thl/Th2的影响。方法 31例RSA患者进行联合淋巴细胞免疫、免疫球蛋白、阿司匹林治疗,测定治疗前后外周血INF-γ、IL-10含量,计算Thl/Th2指标。结果治疗后INF-γ较治疗前明显下降,IL-10较治疗前明显上升,Thl/Th2比值较治疗前明显下降,差异均有统计学意义(P<0.01)。结论 RSA患者存在Thl/Th2平衡异常,联合免疫治疗可诱导Thl向Th2转移,恢复Thl/Th2平衡。

Thl／Th2细胞因子在角膜移植免疫排斥反应中的研究进展

据统计我国因角膜病而致盲者有200～300万人，角膜病成为我国第2大致盲原因。目前治疗角膜病致盲的有效方案当属同种异体角膜移植，但移植术后免疫排斥反应是导致角膜移植失败的首要原因，尤其在高危角膜移植（新生血管、多次角膜移植及活动性炎症）免疫排斥反应可高达50％以上。因此，预防角膜移植排斥反应发生是角膜移植成功的关键。

慢性乙型肝炎在拉米呋定治疗过程中IL－12诱导的THl／TH2细胞因子反应

目的：探讨慢性乙型肝炎在拉米呋定治疗过程中IL—12对PBMC产生THI／TH2细胞因子的影响。方法：在拉米呋定治疗前和治疗3mo、6mo、9mo后，20例慢性乙型肝炎的PBMC在PHA(100μg·mL^-1)、HBcAg(1μg·mL^-1)、habeas(1μg·mL^-1)单独或联合IL—12(10ng·mL^-1)刺激下体外培养48h，收集上清液，用ELIS检测：IFN-γ和IL-10的水平。结果：在拉米呋定治疗3mo后，无论是抗原单独诱导还是联合IL-12共同诱导，PBMC产生-IFN-γ的水平同治疗前相比无显著变化；在治疗6mo后，抗原单独诱导产生IFN-γ的水平同治疗前相比无显著性差异，但IL-12诱导产生IFN-γ的增殖效应明显加强；在治疗9mo后，无论是抗原单独诱导还是联合IL-12共同诱导，PBMC产生IFN-γ的水平同治疗前相比均显著增高，同时IL-10的水平也显著降低。在治疗同一阶段，抗原联合IL-12诱导组产生IFN-γ水平明显高于抗原单独诱导组。结论：拉米呋定治疗慢性乙型肝炎过程中，随着HBV DNA的抑制，IL-l2对乙型肝炎患者PBMC产生IFN-γ协同效应逐渐增强，对IL-10的产生有抑制作用，提示拉咪呋定联合IL-12可能提高慢性乙型肝炎的疗效。

ECT2通过调控PI3K/AKT信号通路对胰腺癌细胞恶性行为、糖酵解及TH细胞分化的影响

目的探讨上皮细胞转化序列2(ECT2)通过调控PI3K/AKT信号通路对胰腺癌细胞恶性行为、糖酵解及TH细胞分化的影响。方法RT⁃qRCR检测人脐静脉内皮细胞系HUVEC及胰腺癌细胞中ECT2 mRNA表达,将胰腺癌Panc⁃1细胞株分为胰腺癌组(Panc⁃1细胞株正常培养)、NC组(Panc⁃1细胞株转染ECT2阴性对照)、ECT2 siRNA组(Panc⁃1细胞株转染ECT2 siRNA)、抑制剂组(Panc⁃1细胞株转染加入PI3K/AKT抑制剂LY294002),ECT2 siRNA+抑制剂组(Panc⁃1细胞株转染ECT2 siRNA加入PI3K/AKT抑制剂LY294002),采用RT⁃qRCR各组细胞中ECT2 mRNA表达;Transwell法检测各组Panc⁃1细胞侵袭能力;划痕实验检测迁移;流式细胞仪检测各组细胞IFN⁃γ及IL⁃4表达;免疫印迹分别检测糖酵解代表蛋白及PI3K/AKT表达。结果胰腺癌组、NC组、ECT2 siRNA组、抑制剂组及ECT2 siRNA+抑制剂组的ECT2 mRNA比较分别为1.00±0.00、0.95±0.03、0.41±0.08、0.65±0.05及0.20±0.04,组间比较,差异有统计学意义(F=310.700,P<0.05);胰腺癌组、NC组、ECT2 siRNA组、抑制剂组及ECT2 siRNA+抑制剂组Panc⁃1细胞侵袭数目分别为(256.30±28.36)个、(241.18±24.05)个、(155.48±17.56)个、(178.90±18.44)个及(95.15±12.10)个,组间比较,差异有统计学意义(F=59.310,P<0.01);胰腺癌组、NC组、ECT2 siRNA组、抑制剂组及ECT2 siRNA+抑制剂组Panc⁃1细胞迁移距离分别为(14.02±1.36)mm、(13.42±1.29)mm、(9.25±0.85)mm、(8.50±0.45)mm及(4.25±0.53)mm,组间比较差异有统计学意义(F=101.200,P<0.05);ECT2 siRNA组细胞IFN⁃γ升高及IL⁃4占比降低,与NC组比较,差异有统计学意义(P<0.05),与抑制剂组相比,ECT2 siRNA+抑制剂组细胞IFN⁃γ升高及IL⁃4占比降低,组间比较差异有统计学意义(P<0.05);ECT2 siRNA组细胞HIF⁃1α、GLUT1、HK⁃Ⅱ和PFK蛋白均降低,与抑制剂组无意义(P>0.05),与抑制剂组相比,ECT2 siRNA+抑制剂组细胞HIF⁃1α、GLUT1、HK⁃Ⅱ和PFK蛋白降低,组间比较差异有统计学意义(P<0.05);ECT2 siRNA组细胞HIF⁃1α、GLUT1、HK⁃Ⅱ和PFK蛋白均降低,与NC组差异有统计学意义(P<0.05),与抑制剂组相比,ECT2 siRNA+抑制剂组细胞HIF⁃1α、GLUT1、HK⁃Ⅱ和PFK蛋白降低,组间比较差异有统计学意义(P<0.05)。结论抑制ECT2可通过降低胰腺癌细胞糖酵解,提高Th细胞中IFN⁃γ表达而抑制恶性侵袭及迁移,其机制可能与抑制PI3K/AKT信号通路活性相关。

妊娠期尖锐湿疣患者外周血Thl/Th2型细胞因子的表达及相关机制研究

目的:针对妊娠期尖锐湿疣(CA)患者外周血Thl/Th2型细胞因子的表达及相关机制展开研究,为临床治疗提供一定的依据。方法:选取我院2011年12月至2012年12月间收治的30例处于妊娠期的尖锐湿疣患者作为本次的研究对象,即妊娠期尖锐湿疣组,并将其与另外30例非妊娠的尖锐湿疣患者进行比较,即非妊娠尖锐湿疣组。采用双抗体夹心ELLSA法检测妊娠期尖锐湿疣患者的血清白细胞介素-2(IL-2)与白细胞介素-10(IL-10)的表达,并将其与正常妊娠患者进行对比。结果:经过研究发现,妊娠期尖锐湿疣组血清IL-2的浓度明显低于与非妊娠尖锐湿疣组相比,两组对比有明显差异(P<0.05)。结论:妊娠可能会通过削弱患者的Th1型反应导加重患者的病情,而尖锐湿疣可能不会影响正常妊娠的母体免疫。

Rapamycin ameliorates experimental autoimmune uveoretinitis by inhibiting Th1/Th2/Th17 cells and upregulating CD4+CD25+ Foxp3 regulatory T cells

· AIM: To determine the effects of rapamycin on experimental autoimmune uveoretinitis(EAU) and investigate of role of rapamycin on T cell subsets in the disease.·METHODS: EAU was induced in rats using peptides1169 to 1191 of the interphotoreceptor binding protein(IRBP). Rapamycin(0.2 mg/kg/d) was administrated by intraperitoneal injection for a consecutive 7d after immunization. Th1/Th2/Th17 cytokines, TGF-β1, and IL-6produced by lymphocyteswere measured by ELISA, while Th17 cells and CD4 +CD25 + regulatory T cells(Tregs)from rat spleen were detected by flow cytometry.·RESULTS: Intraperitoneal treatment immediately after immunization dramatically ameliorated the clinical course of EAU. Clinical responses were associated with reduced retinal inflammatory cell infiltration and tissue destruction. Rapamycin induced suppression of Th1/Th2/Th17 cytokines, including IFN-γ, IL-2, IL-17, IL-4, and IL-10 release from T lymphocytes of EAU rats, in vitro.Rapamycin also significantly increased TGF-β1production but had no effect on IL-6 productionof T lymphocytes from EAU rats in vitro. Furthermore,rapamycin decreased the ratio of Th17 cells/CD4 +T cells and upregulated Tregs in EAU, as detected by flow cytometry.·CONCLUSION: Rapamycin effectively interferes with T cell mediated autoimmune uveitis by inhibiting antigen-specific T cell functions and enhancing Tregs in EAU.Rapamycin is a promising new alternative as an adjunct corticosteroid-sparing agent for treating uveitis.

All-transRetinoic Acid Regulates Th1/Th2 Balance in CD4+T cells When GATA-3 is Deficient

The essential effect of vitamin A on immune function occurs through various mechanisms including direct effect on ThloTh2 balance modulation. However, it is unclear whether or not vitamin A can regulate Thl-Th2 balance under a strong Thl-polarizing condition. Therefore, the purpose of our study was to examine the effect of vitamin A metabolite allotrans retinoic acid （ATRA） on ThloTh2 differentiation in CD4~ T cells under GATA-3 deficiency, which can induce Thl-polarizing condition. In the present study, GATA-3 deficiency T cells were induced by siRNA and checked by real-time quantitative PCR and western blot. GATA-3 deficiency CD4＋ T cells and normal CD4＋ T were treated for 48 h with or without ATRA.

Activated rat hepatic stellate cells influence Th1/Th2 profile in vitro

AIM: To investigate the effects of activated rat hepatic stellate cells(HSCs) on rat Th1/Th2 profile in vitro.METHODS: Growth and survival of activated HSCs and CD4+ T lymphocytes cultured alone or together was assessed after 24 or 48 h. CD4+ T lymphocytes were then cultured with or without activated HSCs for 24 or 48 h and the proportion of Th1 [interferon(IFN)-γ+] and Th2 [interleukin(IL)-4+] cells was assessed by flow cytometry. Th1 and Th2 cell apoptosis was assessed after 24 h of co-culture using a caspase-3 staining procedure. Differentiation rates of Th1 and Th2 cells from CD4+ T lymphocytes that were positive for CD25 but did not express IFN-γ or IL-4 were also assessed after 48 h of co-culture with activated HSCs. Galectin-9 expression in HSCs was determined by immunofluorescence and Western blotting. ELISA was performed to assess galectin-9 secretion from activated HSCs.RESULTS: Co-culture of CD4+ T lymphocytes with activated rat HSCs for 48 h significantly reduced the proportion of Th1 cells compared to culture-alone conditions(-1.73% ± 0.71%; P < 0.05), whereas the proportion of Th2 cells was not altered; the Th1/Th2 ratio was significantly decreased(-0.44 ± 0.13; P < 0.05). In addition, the level of IFN-γ in Th1 cells wasdecreased(-65.71 ± 9.67; P < 0.01), whereas the level of IL-4 in Th2 cells was increased(82.79 ± 25.12; P < 0.05) by co-culturing, as measured by mean fluorescence intensity by flow cytometry. Apoptosis rates in Th1(12.27% ± 0.99%; P < 0.01) and Th2(1.71% ± 0.185%; P < 0.01) cells were increased 24 h after co-culturing with activated HSCs; the Th1 cell apoptosis rate was significantly higher than in Th2 cells(P < 0.01). Galectin-9 protein expression was significantly decreased in HSCs only 24 h after coculturing(P < 0.05) but not after 48 h. Co-culture for 48 h significantly increased the differentiation of Th1 and Th2 cells; however, the increase in the proportion of Th2 cells was significantly higher than that of Th1 cells(1.85% ± 0.48%; P < 0.05).CONCLUSION: Activated rat HSCs lower the Th1/Th2 profile, inhibiting the Th1 response and enhancing the Th2 response, and this may be a novel pathway for liver fibrogenesis.

Integration of scRNA-Seq and Bulk RNA-Seq to analyze the heterogeneity ofcolorectal cancer immune cells and establish a molecular risk model

Background:Colorectal cancer(CRC)is a highly heterogeneous malignant tumor that significantly impacts clinical diagnosis and treatment.Single-cell RNA sequencing is an innovative method for exploring tumor heterogeneity and understanding its role at cellular and genetic levels.Method:The colorectal cancer Single-cell RNA sequencing data were analysed on the immune.RNA-seq data in bulk form was utilized to assess the major genes of the immune cell subsets linked to CRC.We conducted an analysis of the abundance of immune cells in the microenvironment of CRC,and also performed weighted gene co-expression network analysis.Gene set enrichment analysis helped perform two analytical procedures of subtype groups.Furthermore,Least absolute shrinkage and selection operator regression was employed to analyse and screen for a gene signature.Finally,quantitative PCR Was performed to detect the expression levels of signature genes in CRC.Results:The Single-cell RNA sequencing(GSE146771)dataset was integrated to obtain 9 cell clusters.The Single-sample gene set enrichment analysis showed that the related gene expression of T-cell subsets of different functional statuses could vary greatly between patients with GSE146771.Immune cell analysis of TCGA-CRC indicated an improved overall survival rate for patients with elevated Th2 cell abundance.Five-gene signature(Risk Score=-0.205×CDC25C-0.231×GSTCD-0.010×KPNA2-0.002×KIF15-0.171×ORC1)was developed by weighted correlation network analysis,and lasso Cox regression.Then,the risk prediction efficacy of the signature was validated in four GSE datasets.Furthermore,the expression of five genes was reduced in CRC tissue by quantitative PCR.Conclusion:Five-gene signature based on CRC heterogeneity was developed as a prognosis predictor,which can serve as a potential treatment target.

慢性阻塞性肺疾病急性加重患者Thl/Th2细胞因子谱的变化

目的研究Th1/Th2细胞因子谱在慢性阻塞性肺疾病急性加重(AECOPD)患者中的变化。方法该次研究抽取的以30例慢性阻塞性肺疾病急性加重患者、30例慢性阻塞性肺疾病稳定者和30名健康者作为研究对象,其入院时间为2013年1—12月。用流式微球阵列分析术(CBA)检测各组Th1/Th2细胞因子包括IL-4、IL-6、IL-10、TNF-α、IFN-γ的表达水平。结果 AECOPD组血清产生IL-4(27.22±1.51)pg/mL、IL-6(47.73±4.72)pg/mL低于慢性阻塞性肺疾病稳定组(34.79±1.37)、(72.38±5.31)pg/mL,(P<0.05)。AECOPD组血清产生IL-10(35.76±2.56)pg/mL低于慢性阻塞性肺疾病稳定组(45.15±2.08)pg/mL,(P<0.05)。AECOPD组血清产生TNF-α(19.11±1.08)pg/mL、IFN-γ(40.33±3.69)pg/mL高于慢性阻塞性肺疾病稳定组(12.93±0.36)、(22.28±1.16)pg/mL,(P<0.05)。而慢性阻塞性肺疾病稳定组其IL4(34.79±1.37)pg/mL、IL-6(72.38±5.31)pg/mL、IL-10(45.15±2.08)pg/mL、TNF-α(12.93±0.36)pg/mL、IFN-γ(22.28±1.16)pg/mL的表达水平与健康对照组(33.72±1.66)、(67.06±6.89)、(43.84±2.45)、(13.81±0.38)、(23.59±1.21)pg/mL相比,均差异无统计学意义(P>0.05)。结论慢性阻塞性肺疾病急性加重患者存在Thl/Th2细胞因子失衡。

Effects of the Overall Alkaloid of a Traditional Chinese Medicine “Tongbiling” on the Cytokine Expression in Th1 and Th2 Cells of Rheumatoid Arthritis and Their Signaling Pathway

To investigate the effects of overall alkali of a traditional Chinese medicine “Tongbiling” (brucine and strychnine alkaloids in main) on the cytokines expression in Th1 and Th2 cells in the synovial fluid of patients with rheumatism arthritis and their signal pathway, the mononuclear cells in the synovial fluid (SFMC) of patients were isolated by Ficoll-Hypaque gradient centrifugation, and the CD3 + CD69 + and CD3 + HLA-DR antigen were analyzed by flow cytometry in comparison with those of the peripheral blood. The rest of cells were cultured after resuspension with RPMI 1640 culture medium. Phorbol 12,13-dibutyrate (PDB) and ionomycin were added successively into the culture with various concentration of overall alkali Tongbiling (TBL). After 4 h of cultivation, the expression of IFN-γ and IL-4 in CD3 + cells were analyzed by flow cytometry. The influence of overall alkali TBL (100?mg/L) on the intracellular calcium was investigated after Fluo-3/AM labeling and stimulation with PDB and ionomycin at 1, 2, 4 and 10?min, and the influence of TBL on the expression of CD3 + CD69 + cells were determined with stimulation of PDB for 24?h in the whole blood lymphocytes culture. It was found that the percentage of T cells bearing CD69 was significantly up-regulated (77%), while that of T cells bearing HLA-DR was 44% in the synovial mononucleated cells. After PDB and ionomycin stimulation, the expression of IFN-γ in CD3 + cells were up-regulated, but there was no change on the expression of IL-4 in CD3 + cells, indicating that ratio of Th1/Th2 was significantly increased and Th cells differentiate to Th1 cells in mainly. Four concentrations of overall alkaloid of TBL (200?mg/L, 100?mg/L, 50?mg/L, 25?mg/L) could down-regulated the expression of IFN-γ in CD3 + cells and the Th1/Th2 ratio obviously, but all the concentrations of the overall alkaloids had no effect on the expression of IL-4 in CD3 + cells. 100?mg/L concentration of the overall alkaloid did not down-regulate the intracellular calcium level. Each concentration of the overall alkaloid could down-regulated the expression CD69 obviously on the PDB-activated mouse T cells. It concluded from the above observations that the overall alkaloid of TBL could relieve the inflammatory and immune damages by suppressing the expression of Th1 type cytokines and Th1 cell differentiation, regulating the imbalance of Th1/Th2 cells and inhibiting the early activation of the T lymphocytes bearing CD69. There was no remarkable influence on the intracellular calcium signaling transduction pathway. The inhibitory effected on T cells to express IFN-γ might be due to the suppression of PKC-MAPK signaling pathway. From the standpoint of traditional Chinese medicine, this might be due to the regulation of “Yin” and “Yang” imbalance of joints to modify the pathological status in rheumatoid arthritis. This study provided an experimental basis for the application of overall alkaloids of TBL in the treatment of rheumatoid arthritis.

T-Helper I Cell/T-Helper 2 Cell Balance with Anti Inflammatory Therapy in Partly Controlled Asthmatic Children

The authors aimed to assess Thl （T-helper cell 1）/Th2 （T-helper cell 2） balance, through evaluation of serum IFN-γ （interferon gamma） and IL-4 （interleukin 4）, during asthma exacerbation and study the effect of anti inflammatory therapy. A randomized prospective case-control study was designed. The sludy included 30 asthmatic patients, aging 8-14 years. All were diagnosed as partly controlled asthmatics. Twenty, age and sex matched, healthy children were included in the study as control group All participants were subjected to medical history, clinical examination, pulmonary function testing, eosinophilic blood counting, estimation of serum interleukine-4 and interferon gamma. Patients were treated for 6 weeks with 2 different anti inflammatory drugs. All methods were then repeated for follow up. IL-4 serum level was significantly higher in subjects with partly controlled asthma than in control subjects （P = 0.01）, and then in asthmatic patients after therapy （P = 0.0000）, while IFN-）, serum level was significantly lower in subjects with partly controlled asthma than in control subjects （P = 0.01）, and than in asthmatic patients after therapy （P = 0.0000）. Interferon gamma showed a significant negative correlation with IL-4 among the healthy control group （r = -0.559, P = 0.010）. Both LTA （leukotriene antagonist） and ICS （inhaled corticosteroids） therapy lead to significant improvement, but there were no statistically significant differences （P 〉 0.05） between them as regard the pulmonary functions and the laboratory evaluating parameters. Both serum levels of IL-4 and IFN-γ, could be used as a reliable inflammatory biomarker for the evaluation and follow up of asthmatic patients.

CD_4^(+) EFFECTOR CELLS DEFAULT TO THE TH2 PATHWAY IN INTERFERONγ-DEFICIENT MICE INFECTED WITH LEISHMANIA MAJOR

Mice with homologous disruption of the interferon γ(IFN-γ) gene on the C57BL/6 background were infected witly Leishmania major and the immune response assessed. In contrast to wild-type or heterozygous knockout mice,deficient animals were unable to restrict growth of the parasite and suffered lethal infection over 6￣8 wk.Although wild-type and heterozygous littermates developed CD4+ cells that contained transcripts for IFN-γ and lymphotoxin,tipical of T helper type 1(Th1) cells, the knockout mice developed CD+4 cells that contained transcripts for interleukin 4(IL-4),IL-5,and IL13,typical of Th2 cells. ELISPOT assays confirmed the reciprocal patterns of IFN-γ or IL-4 production by T cells in similar frequencies in the respective groups of mice,and antibody analysis confirmed the presence of Th2-mediated isotype switching in the knockout mice. These data suggest that CD4+ T cells that normally respond to antigens by differentiation to Th1 cells default to the Th2 pathway in the absence of endogenous IFN-γ.

Impact of Bisphenol A (BPA) and Free Fatty Acids (FFA) on Th2 Cytokine Secretion from INS-1 Cells

Bisphenol A (BPA) is used in huge amounts for many plastic products and is a hormone (estrogen) disrupting agent. BPA as well as FFAs may be deleterious for the immune system. The aim was to identify Th2 cytokines and some of their signal transduction mechanisms in INS-1 cells, an insulin secreting cell line. Screening using a proteome profile indicated an increase of IL-1, IL-2, IL-4, IL-6, IL-10, IL-13 and IL-17 by BPA. Also FFAs (in combination with LPS) were positive. In detailed quantitative measurements, these results were confirmedly indicating a complex array of pro-and anti-inflammatory potential. The interaction of BPA with 17β-estradiol was non-additive with respect to IL-4 and IL-6 release and additive with respect to FFA interaction indicating same and different mechanisms of action, respecttively. As signal transduction PI3K (Wortmannin-sensitive) and STAT-3/6 (Tofacitinib-sensitive) are involved in various effects, INS-1 cells release several cytokines due to BPA and FFA attack which may be involved in disturbance of glucose homoeostasis and type 1 diabetes.

Silencing of <i>ERK2</i>with Small Interference RNA Regulates the Expression of CXCL1 in Th17 Cell

Patients with steroid-resistant asthma had their monocyte-derived TH17 cells collected. The expression levels of ERK2 in the TH17 were silenced and inhibited using ERK2 specific small interfering RNA (siRNA). By screening of CXCL1 and IL-17A in the TH17 culture supernatant, the expression levels of ERK2 and CXCL1 were determined. Using targeted siRNA to inhibit ERK2, the expression of ERK2 in the TH17 was reduced. Furthermore, inhibiting ERK2 hindered CXCL1 expression and decreased CXCL1 and IL-17A production. These findings suggest that ERK2 is involved in the synthesis of CXCL1 and IL-17A, two proteins that play a key role in the pathogenesis of hormone-resistant asthma.