Correlation between CD4^＋CD25^＋Treg Cells and CCR4 in Nasopharyngeal Carcinoma

OBJECTIVE CD4^＋CD25^＋ T regulatory （Treg） cells are a population of T cells which suppress an overactive immune system. CCR4 is a chemokine receptor involved in the recruitment of lymphocytes. Nasopharyngeal carcinoma （NPC） is resistant to immunosurveillance, owing to the increased number of tumor-infiltrating Treg cells which are recruited to the tumor bv CCR4.

新型调节性T细胞CD4^+LAP^+ Treg与疾病的研究进展

调节性T细胞(Treg)是体内存在的一类抑制免疫应答的T细胞亚群,分为天然调节性T细胞(CD4+CD25+Treg)和诱导型调节性T细胞(iTreg),通过细胞-细胞互相接触、分泌细胞因子(IL-10、TGF-β1)等途径抑制B细胞、效应性T细胞的增殖、活化和免疫效应,在抑制自身免疫性疾病发展、移植耐受、肿瘤免疫逃逸等方面发挥重要作用。新的调节性T细胞亚群:CD4+LAP+调节性T细胞(CD4+LAP+Treg),已经被证实在多种动物模型中发挥保护作用,可能是Treg发挥免疫抑制功能关键细胞之一,目前已引起国内外学者的关注。本文对CD4+LAP+Treg的发现及其与疾病关系的研究进展进行综述。

Effects of GW5074 in the process of imDCs inducing differentiation of naive CD4^+ T cells into Treg cells in vitro

Objective To establish a stable and efficient method of culturing imDCs in vitro,and to explore the effect of GW5074,which blocks ERK1 /2 signal pathway in the process of immature dentritic cells ( imDCs) on inducing differentiation of the naive allogeneic CD4 + T

An Association between Immunosenescence and CD4^+CD25^+ Regulatory T Cells: A Systematic Review

Objective Age-related increment of the prevalence of CD4^＋CD25^＋ regulatory T （Treg） cells were described controversially, and whether such changes explain immune dysfunction in the elderly is still unclear. The aim of this systematic review is to evaluate the role of the Tregs in immunosenescence. Methods Medline and manual searches were performed to identify all published epidemiological and animal studies investigating the efficacy of the association between immunosenescence and Treg cells. Results It was founded that the frequency, phenotypic characteristics, and number/function of Tregs were altered significantly with aging. Medical conditions in individuals with advanced ageas well as apoptosis intensity of Treg cells had an impact on the accumulation of Tregs which in turn could deteriorate cytotoxic activity of CD8＋ T and NK cells and production of IL-2. The range of immune cells that could be suppressed by Treg cells was quite wide and covered CD4^＋CD25^＋ T cells, NK cells, dendritic cells and even monocytes. These changes were observed both in humans and experimental animals. Besides, it was believed that frequency of Tregs increased with age and was accompanied by intensified suppressive activity for Tregs in patients, for example, with Alzheimer disease （AD） and Parkinson disease （PD）. The impaired condition of CD4＋ T cells, so-called immunosenescence, rendered transplant recipients less responsive to an allogeneic kidney graft, an effect that was limited to transplant recipients who were aged over 60 years. Conclusions Treg cells are associated with immunosenescence. All these changes contribute to the aging-related decline of immune responses and lead to the higher risk of immune-mediated diseases, cancer or infections in aged individuals.

Downregulation of CD4+CD25+ regulatory T cells may underlie enhanced Th1 immunity caused by immunization with activated autologous T cells

Regulatory T cells （Treg） play important roles in immune system homeostasis, and may also be involved in tumor immunotolerance by suppressing Th1 immune response which is involved in anti-tumor immunity. We have previously reported that immunization with attenuated activated autologous T cells leads to enhanced anti-tumor immunity and upregulated Thl responses in vivo. However, the underlying molecular mechanisms are not well understood. Here we show that Treg function was significantly downregulated in mice that received immunization of attenuated activated autologous T cells. We found that Foxp3 expression decreased in CD4＋CD25＋ T cells from the immunized mice. Moreover, CD4＋CD25＋Foxp3＋ Treg obtained from immunized mice exhibited diminished immunosuppression ability compared to those from naive mice. Further analysis showed that the serum of immunized mice contains a high level ofanti-CD25 antibody （about 30 ng/ml, p〈0.01 vs controls）. Consistent with a role ofanti-CD25 response in the downregulation of Treg, adoptive transfer of serum from immunized mice to naive mice led to a significant decrease in Treg population and function in recipient mice. The triggering of anti-CD25 response in immunized mice can be explained by the fact that CD25 was induced to a high level in the ConA activated autologous T cells used for immunization. Our results demonstrate for the first time that immunization with attenuated activated autologous T cells evokes anti-CD25 antibody production, which leads to impeded CD4＋CD25＋Foxp3＋ Treg expansion and function in vivo. We suggest that dampened Treg function likely contributes to enhanced Thl response in immunized mice and is at least part of the mechanism underlying the boosted anti-tumor immunity.

Heterogeneity and plasticity of T helper cells

CD4 T helper （Th） cells play critical roles in adaptive immune responses. They recruit and activate other immune cells including B cells, CD8 T cells, macrophages, mast cells, neutrophils, eosinophils and basophils. Based on their functions, their pattern of cytokine secretion and their expression of specific transcription factors, Th cells, differentiated from naive CD4 T cells, are classified into four major lineages, Thl, Th2, Th17 and T regulatory （Treg） cells, although other Th lineages may exist. Subsets of the same lineage may express different effector cytokines, reside at different locations or give rise to cells with different fates, whereas cells from different lineages may secrete common cytokines, such as IL-2, IL-9 and IL-10, resulting in massive heterogeneity of the Th cell population. In addition, the pattern of cytokine secretion may switch from that of one lineage toward another under certain circumstances, suggesting that Th cells are plastic. Tregs are also more heterogeneous and plastic than were originally thought. In this review, we summarize recent reports on heterogeneity and plasticity of Th cells, and discuss potential mechanisms and implications of such features that Th cells display.

Treg/Th17 cell balance and phytohaemagglutinin activation of T lymphocytes in peripheral blood of systemic sclerosis patients

AIM To investigate T-cell activation, the percentage of peripheral T regulatory cells(Tregs), Th17 cells and the circulating cytokine profile in systemic sclerosis(SSc).METHODS We enrolled a total of 24 SSc patients and 16 healthy controls in the study and divided the patients as having diffuse cutaneous SSc(dc SSc, n = 13) or limited cutaneous SSc(lc SSc, n = 11). We performed a further subdivision of the patients regarding the stage of the disease-early, intermediate or late. Peripheral venous blood samples were collected from all subjects. We performed flow cytometric analysis of the activationcapacity of T-lymphocytes upon stimulation with PHA-M and of the percentage of peripheral Tregs and Th17 cells in both patients and healthy controls. We used ELISA to quantitate serum levels of human interleukin(IL)-6, IL-10, tissue growth factor-β1(TGF-β1), and IL-17 A.RESULTS We identified a decreased percentage of CD3+CD69+ cells in PHA-stimulated samples from SSc patients in comparison with healthy controls(13.35% ± 2.90% vs 37.03% ± 2.33%, P < 0.001). However, we did not establish a correlation between the down-regulated CD3+CD69+ cells and the clinical subset, nor regarding the stage of the disease. The activated CD4+CD25+ peripheral lymphocytes were represented in decreased percentage in patients when compared to controls(6.30% ± 0.68% vs 9.36% ± 1.08%, P = 0.016). Regarding the forms of the disease, dc SSc patients demonstrated lower frequency of CD4+CD25+ T cells against healthy subjects(5.95% ± 0.89% vs 9.36% ± 1.08%, P = 0.025). With regard to Th17 cells, our patients demonstrated increased percentage in comparison with controls(18.13% ± 1.55% vs 13.73% ± 1.21%, P = 0.031). We detected up-regulated Th17 cells within the lc SSc subset against controls(20.46% ± 2.41% vs 13.73% ± 1.21%, P = 0.025), nevertheless no difference was found between dc SSc and lc SSc patients. Flow cytometric analysis revealed an increased percentage of CD4+CD25-Foxp3+ in dc SSc patients compared to controls(10.94% ± 1.65% vs 6.88% ± 0.91, P = 0.032). Regarding the peripheral cytokine profile, we detected raised levels of IL-6 [2.10(1.05-4.60) pg/m L vs 0.00 pg/m L, P < 0.001], TGF-β1(19.94 ± 3.35 ng/m L vs 10.03 ± 2.25 ng/m L, P = 0.02), IL-10(2.83 ± 0.44 pg/m L vs 0.68 ± 0.51 pg/m L, P = 0.008), and IL-17 A [6.30(2.50-15.60) pg/m L vs 0(0.00-0.05) pg/m L, P < 0.001] in patients when compared to healthy controls. Furthermore, we found increased circulating IL-10, TGF-β, IL-6 and IL-17 A in the lc SSc subset vs control subjects, as it follows: IL-10(3.32 ± 0.59 pg/m L vs 0.68 ± 0.51 pg/m L, P = 0.003), TGF-β1(22.82 ± 4.99 ng/m L vs 10.03 ± 2.25 ng/m L, P = 0.031), IL-6 [2.08(1.51-4.69) pg/m L vs 0.00 pg/m L, P < 0.001], and IL-17 A [14.50(8.55-41.65) pg/m L vs 0.00(0.00-0.05) pg/m L, P < 0.001]. Furthermore, circulating IL-17 A was higher in lc SSc as opposed to dc SSc subset(31.99 ± 13.29 pg/m L vs 7.14 ± 3.01 pg/m L, P = 0.008). Within the dc SSc subset, raised levels of IL-17 A and IL-6 were detected vs healthy controls: IL-17 A [2.60(0.45-9.80) pg/m L vs 0.00(0.00-0.05) pg/m L, P < 0.001], IL-6 [2.80(1.03-7.23) pg/m L vs 0.00 pg/m L, P < 0.001]. Regarding the stages of the disease, TGF-β1 serum levels were increased in early stage against late stage, independently from the SSc phenotype(30.03 ± 4.59 ng/m L vs 13.08 ± 4.50 ng/m L, P = 0.017).CONCLUSION It is likely that the altered percentage of Th17 and CD4+CD25-Fox P3+ cells along with the peripheral cytokine profile in patients with SSc may play a key role in the pathogenesis of the disease.

Magnetic cell sorting and flow cytometry sorting methods for the isolation and function analysis of mouse CD^4+ CD25^+ Treg cells

Objective: In this paper we compared the two methods of cell sorting (magnetic cell sorting and flow cytometry sorting) for the isolation and function analysis of mouse CD4+ CD25+ regulatory T (Treg) cells, in order to inform further studies in Treg cell function. Methods: We separately used magnetic cell sorting and flow cytometry sorting to identify CD4+ CD25+ Treg cells. After magnetic cell separation, we further used flow cytometry to analyze the purity of CD4+ CD25+ Treg cells, trypan blue staining to detect cell viability, and propidium iodide (PI) staining to assess the cell viability. We detected the immune inhibition of CD4+ CD25+ Treg cells in the in vitro proliferation experiments. Results: The results showed that compared to flow cytometry sorting, magnetic cell sorting took more time and effort, but fewer live cells were obtained than with flow cytometry sorting. The CD4+ CD25+ Treg cells, however, obtained with both methods have similar immunosuppressive capacities. Conclusion: The result suggests that both methods can be used in isolating CD4+ CD25+ Treg cells, and one can select the best method according to specific needs and availability of the methodologies.

维吾尔族宫颈癌患者手术前后HPV感染与Th17/Treg细胞的相关性

目的探讨维吾尔族宫颈癌患者手术前后人乳头瘤病毒(HPV)与外周血CD+4IL17+Th17细胞、CD+4CD+25调节性T(Treg)细胞、IL-6、IL-23、IL-17、TGF-β、IL-10细胞因子的相关性。方法收集2014年12月-2015年12月就诊新疆医科大学第一附属医院妇科宫颈HPV感染的维吾尔族宫颈病变患者共60例,宫颈癌(CC组)30例,子宫上皮内瘤变(CINⅡ~Ⅲ组)30例。分别于手术前及手术3个月后检测宫颈HPV、外周血T细胞亚群(CD+4CD+25Treg细胞、CD+4IL17+Th17细胞的含量)、血清IL-6、IL-23、IL-17、TGF-β、IL-10的表达水平。HPV检测采用HPV核酸扩增分型检测试剂盒,T细胞亚群采用流式细胞仪技术,酶联免疫吸附剂测定(ELISA)检测相关细胞因子。结果 (1)手术治疗CC及CINⅡ~Ⅲ患者后HPV转阴明显升高,CC组HPV转阴率为60%,CINⅡ~Ⅲ组HPV转阴率为53%;(2)CC组和CINⅡ~Ⅲ组手术后外周血CD+4IL17+Th17%、CD+4CD+25Treg%、Th17/Treg比率及相关细胞因子均低于手术前,差异有统计学意义(P<0.01);(3)CC组与CINⅡ~Ⅲ组对照,术前及术后CD+4IL17+Th17%、CD+4CD+25Treg%、Th17/Treg比率CC组高于CINⅡ~Ⅲ组;(4)术后HPV持续阳性的CC患者外周血CD+4CD+25Treg%、CD+4IL17+Th17%及Th17/Treg比率表达水平高于术后HPV转阴的CC患者,差异有统计学意义(P<0.05)。结论手术治疗宫颈癌及子宫颈上皮内瘤变后,宫颈HPV的感染率、CD+4CD+25Treg细胞、CD+4IL17+Th17细胞、Th17/Treg细胞及相关细胞因子降低,Th17/Treg细胞失衡可能直接参与宫颈HPV感染的免疫逃避,并与病情发展相关。术后监测外周血Th17、Treg细胞可能成为宫颈癌患者病情进展及复发的指标之一。

LAP＋CD4＋Treg细胞在结直肠癌患者外周血中的分布及意义

目的探讨LAP＋CD4＋Treg细胞在结直肠癌患者外周血中的分布及其与患者临床病理因素的关系。方法采用回顾性病例对照研究方法。收集2014年4—10月广西医科大学附属第一医院收治的40例行结直肠癌根治术患者和同期20例健康志愿者的临床资料。采用流式细胞仪检测外周血LAP＋CD4＋Treg细胞比例。观察指标：（1）结直肠癌患者及健康志愿者外周血LAP＋CD4＋Treg细胞比例。（2）结直肠癌患者临床病理因素与外周血LAP＋CD4＋Treg细胞比例的关系。（3）对与结直肠癌患者外周血LAP＋CD4＋Treg细胞比例相关的临床病理因素进行进一步定量相关性分析。正态分布的计量资料以z±S表示，组间比较采用t检验。采用Pearson检验进行相关性分析。结果（1）流式细胞仪检测外周血LAP＋CD4＋Treg细胞比例情况：结直肠癌患者外周血LAP＋CD4＋Treg细胞比例为9．4％±2．9％，健康志愿者为1．5％±0．7％，两者比较，差异有统计学意义（i=12．275，P〈0．05）。（2）结直肠癌患者临床病理因素与外周血LAP＋CD4＋Treg细胞比例的关系：血清CEA〈5．0μg／L的结直肠癌患者外周血LAP＋CD4＋Treg细胞比例为8．5％±3．2％，≥5．0μg／L患者为12．3％±3．0％；Dukes分期为A～B期患者为8．1％±1．1％，C～D期患者为10．8％±2．0％；有淋巴结转移的患者为11．4％±2．0％，无淋巴结转移的患者为9．3％±2．1％。不同血清CEA、Dukes分期、淋巴结转移的结直肠癌患者外周血LAP＋CD4＋Treg细胞比例比较，差异均有统计学意义（t=2．783，-5．376，3．276，P〈0．05）。（3）相关性分析：结直肠癌患者血清CEA与外周血LAP＋CD4＋Treg细胞比例呈正相关，差异有统计学意义（r=0．543，P〈0．05）。结论LAP＋CD4＋Treg细胞在结直肠癌患者外周血中比例增加，且不同血清CEA、Dukes分期和淋巴结转移患者，外周血LAP＋CD4＋reg细胞比例不同。患者血清CEA与外周血LAP＋CD4＋Treg细胞比例呈正相关。

2-Gy whole-body irradiation significantly alters the balance of CD4^(+)CD25^(-) T effector cells and CD4^(+)CD25^(+)Foxp3^(+) T regulatory cells in mice

CD4^(+)CD25^(+) T regulatory(Treg)cells are critical in inducing and maintaining immunological self-tolerance as well as transplant tolerance.The effect of low doses of whole-body irradiation(WBI)on CD41CD251Foxp31 Treg cells has not been determined.The proportion,phenotypes and function of CD4^(+)CD25^(+) Treg cells were investigated 0.5,5 and 15 days after euthymic,thymectomized or allogeneic bone marrow transplanted C57BL/6 mice received 2-Gy c-rays of WBI.The 2-Gy WBI significantly enhanced the ratios of CD41CD251 Treg cells and CD4^(+)CD25^(+)Foxp3^(+) Treg cells to CD41 T cells in peripheral blood,lymph nodes,spleens and thymi of mice.The CD41CD251 Treg cells of the WBI-treated mice showed immunosuppressive activities on the immune response of CD4^(+)CD25^(+) T effector cells to alloantigens or mitogens as efficiently as the control mice.Furthermore,2-Gy c-ray WBI significantly increased the percentage of CD4^(+)CD25^(+)Foxp3^(+) Treg cells in the periphery of either thymectomized mice or allogeneic bone marrow transplanted mice.The in vitro assay showed that ionizing irradiation induced less cell death in CD4^(+)CD25^(+)Foxp3^(+) Treg cells than in CD4^(+)CD25^(+) T cells.Thus,a low dose of WBI could significantly enhance the level of functional CD41CD251Foxp31 Treg cells in the periphery of naive or immunized mice.The enhanced proportion of CD41CD251Foxp31 Treg cells in the periphery by a low dose of WBI may make hosts more susceptible to immune tolerance induction.

结直肠癌患者外周血LAP+CD4+调节性T细胞的细胞因子谱分析

目的 LAP+CD4+调节性T细胞(LAP+CD4+Treg)是新近发现的调节性T细胞亚型,在结直肠癌发病机制中的作用尚不完全清楚。本研究通过检测结直肠癌患者外周血中LAP+CD4+Treg的细胞因子谱,探讨其在结直肠癌发病机制中的作用。方法收集2014-11-10-2015-02-01广西医科大学第一附属医院初次手术治疗的32例CRC患者的外周血,采用免疫磁珠法(magnetic cell sorting,MACS)分选出LAP+CD4+Treg细胞以及LAP-CD4+T细胞,并用流式细胞术(flow cytometry,FCM)检测其纯度;台盼蓝掺入法检测其存活率;应用液相芯片(luminex liquichip)、酶联免疫法(enzyme-linked immunosorbent,ELISA)检测两种细胞培养上清液所含相关细胞因子IL-2、IL-4、IL-10、IL-17、干扰素-γ(Interferon-γ,IFN-γ)和转化生长因子-β(transforming growth factor-β,TGF-β)的浓度。结果 MACS分选获得的LAP+CD4+Treg细胞纯度为(95.14±1.67)%,LAP-CD4+T细胞纯度为(95.32±2.41)%;台盼蓝掺入法结果显示,LAP+CD4+Treg细胞存活率为(92.54±2.31)%,分选出的CD4+T细胞后存活率为(93.24±2.41)%,说明分选前后细胞均保持较高存活率,t=1.856,P>0.08;液相芯片以及ELISA检测结果表明,LAP+CD4+Treg细胞较LAP-CD4+T细胞分泌更高浓度的IL-10分别为110.65±12.45和72.86±10.87,t=9.13,P<0.001;TGF-β为107.03±17.69和64.19±14.15,t=7.76,P<0.001。结论 CRC患者外周血LAP+CD4+Treg细胞可能通过分泌高浓度细胞免疫抑制因子IL-10、TGF-β参与了机体肿瘤的免疫逃逸机制。

Value of regulatory T cell in predicting the chronic hepatitis C

Objective:To explore the proportion and clinical predictive value of serum regulatory T cells (CD4+CD25+Treg cell) in the treatment process of chronic hepatitis C (CHC) by the interferon. Methods:A total of 94 patients with CHC who were admitted in our hospital for the treatment of peglyated interferon-α and ribavirin were included in the study and were divided into low, moderate, and high loading capacity groups according to HCV-RNA content before treatment. The correlation of different loading capacity with the clinical materials was analyzed. HCV-RNA and the proportion of peripheral blood CD4+CD25+Treg cells after treatment in patients with different response were detected and compared.Results: The comparison of the proportion of peripheral blood CD4+CD25+Treg cells and HCV-RNA among the three groups was statistically significant (P<0.05), and both of them were positively correlated (r=0.845, P=0.001). Among 94 patients, 90 patients had completed 48-week treatment, among which 55 had continuous response, 25 had partial response, and 10 had no response. The proportion of CD4+CD25+Treg cells in the continuous response group and partial response group was significantly reduced when compared with before treatment (P<0.05), while that in the no response group was significantly elevated when compared with before treatment (P<0.05). The comparison of the proportion of CD4+CD25+Treg cells 24 and 48 weeks after treatment among the three groups was statistically significant (P<0.05). CD3+, CD4+, CD8+, and CD4+/CD8+ after treatment in the continuous response and partial response groups were significantly elevated when compared with before treatment (P<0.05). The comparison of CD3+, CD4+, CD8+, and CD4+/CD8+ among the three groups was statistically significant (P<0.05). Conclusions:Interferon in the treatment of CHC can reduce HCV-RNA loading capacity and the proportion of CD4+CD25+Treg cells. HCV-RNA loading capacity in patients with CHC has no correlation with the gender and age, but is positively correlated with the proportion of peripheral blood CD4+CD25+Treg cells. The change of CD4+CD25+Treg cell level can provide a new thought to predict the efficacy in CHC patients.

MicroRNA-125b regulates Th17/Treg cell differentiation and is associated with juvenile idiopathic arthritis

Background Juvenile idiopathic arthritis(JIA)is the most common rheumatic disease in childhood driven by aberrant pathways of T-cell activation.T helper 17(Th17)/regulatory T cell(Treg)imbalance plays critical roles in the pathogenesis of arthritis.MicroRNA-125b(miR-125b)was upregulated after the activation of the initial CD4^+T cells,and could regulate the differentiation of CD4^+T cells.However,the effects of miR-125b on Th17/Treg imbalance and differentiation of Th 17/Treg cells remain unknown.Methods In this study,we evaluated the expression of miR-125b in the peripheral blood mononuclear cells(PBMCs)of children with JIA,and the relationship of miR-125b with Th17/Treg imbalance.Then,we used lentivirus vector-mediated overexpression technology to investigate the regulatory function of miR-125b in CD4^+T cells or dendritic cell/CD4^+T co-culture system.Results Decreased miR-125b expression in PBMCs and CD4^+T cells of JIA patients was negatively correlated with the ratio of Th17/Treg cells.It also correlated negatively with retinoic acid receptor-related orphan receptorγt but positively with Forkhead box protein 3 at transcriptional levels.Furthermore,we found that miR-125b overexpression inhibited Th17 cell differentiation,whereas facilitated the differentiation of Treg cells.MiR-125b upregulation led to the decrease of Th 17-secreting cytokines but the increase of the Treg-secreting cytokines.Conclusions Our results demonstrate that miR-125b participated in regulating Thl7/Treg cell differentiation and imbalance in JIA patients.These findings provide novel insight into the critical role of miR-125b in the Th17/Treg imbalance of JIA,and raise the distinct possibility that miR-125b may prove to be a potential therapeutic target for JIA.

树突状细胞对Thl7／Treg免疫平衡调节的研究进展

树突状细胞（dendritic cells，DCs）对辅助性T细胞17（Thelp cell 17，Thl7）／调节性T细胞（regu—latory T cell，Treg）平衡的调控是免疫学研究中目前最为活跃的研究领域之一。Treg和新近发现的Thl7是机体存在的两种不同于Thl和Th2的CD4＋T细胞新亚型。Thl7细胞介导炎症、延续破坏进程，Treg细胞对抗炎症、维持免疫耐受。

非霍奇金淋巴瘤患者外周血调节性T细胞检测的临床意义

目的:检测非霍奇金淋巴瘤(non-Hodgkin’s lymphoma,NHL)患者外周血中CD4+CD25+Foxp3+调节性T细胞(regu-latory Tcell,Treg)比例的变化,初步分析其在肿瘤免疫调节中的作用及临床意义。方法:采用FCM法检测42例NHL患者化疗前后外周血中CD4+CD25+/CD4+、CD4+CD25+Foxp3+/CD4+T细胞比例的变化,并与28例健康对照进行比较。结果:NHL患者化疗前外周血中CD4+CD25+/CD4+T细胞的比例为(20.71±4.22)%,CD4+CD25+Foxp3+/CD4+T细胞的比例为(4.45±1.52)%,均明显高于健康对照(P<0.01)。化疗后,NHL患者外周血中CD4+CD25+/CD4+T细胞的比例为(11.32±3.13)%,CD4+CD25+Foxp3+/CD4+T细胞的比例为(2.27±1.07)%,均较化疗前明显降低(P<0.05);但仍高于健康对照,差异有统计学意义(P<0.05)。结论:NHL患者外周血Treg比例升高,可能引起机体免疫抑制,并推测与NHL患者的发病相关。

Roles of FOXP3 in experimental atherosclerosis of ApoE-knockout mice

Background Subtypes of T cells, called regulatory T cells （Treg cell）, play a critical role in limiting autoimmune processes and inflammatory responses, The aim of this study was to explore functional roles of FOXP3 in the manifestation of atherosclerosis in Apolipoprotein E deficient （ApoE）-/- mice. Methods Lentivirus-mediated （siRNA） was used to knock down FOXP3 and FOXP3high＋CD4＋ CD25＋ T cells adoptive transfer assays in high fat diet ApoE-/- mice were done. The resulting atherosclerotie lesions were assessed by determining FOXP3 transcript levels and investigating the expression of FOXP3 protein in different tissues. Results Animals treated with siRNA of FOXP3 showed a significant increase in atherosclerotic lesion formation and a reduction in the number of FOXP3＋CD4＋CD25＋ T cells compared with other groups. Transfer of FOXP3highCD4＋CD25＋ T cells significantly decreased atherosclerotic plaque formation and increased the number of FOXP3＋ CD4＋ CD25＋ T cells. FOXP3 protein levels and FOXP3 transcript levels were lowest in the siRNA group, and were highest in tissues from the Treg transfer group. Conclusion FOXP3 plays an important role in regulating the inflammatory response within the atherosclerotic lesion. It can inhibit significantly the progression of the atherosclerosis plaque in ApoE-/- mice.

Effects of MSCs on the progression of atherosclerosis plaque in ApoE-knockout mice

Background Immune inflammatory response is throughout the entire process of atherosclerosis （AS）. It was unclear whether the mechanism of mesenchymal stem cells （MSCs） transplantation for treatment of AS is involved with inflammation regulation in the plaque area. The aim of this study was to explore the effects of MSCs in the formation of atherosclerosis plaque in hypercholesterolemic apoliprotein （apo）E-/- mice. Methods ApoE-/- mice MSCs were isolated and identified. At 8 weeks of age, 30 male ApoE-/- mice were randomly divided into negative control group （Neg, n = 10）, positive control group （Pos, n = 10） and mesenchymal stem cells group （MSCs, n = 10）. MSCs were injected through caudal vein into the body of Pos and MSCs group. The plaque area of all subjects were compared, the percentage of CD4^＋CD25^＋Tregs in different tissues were analyzed by fluorescence activated cell sorter （FACS）, proliferation response of splenocytes to MSCs was detected and cytokines in the supernatant were determined by enzyme linked immunosorbent assay （ELISA）. Results Compared with controls, MSCs resulted in a significant decrease of latherosclerotic plaques size （P 〈 0.05）, and a significant increase of CD4^＋CD25^＋ regulatory T cells in spleen （P 〈 0.05）. Specific proliferation response of CD4^＋CD25^＋ regulatory T cells in splenocytes to MCSs was significantly suppressed, the superanant level of TGF-[3 and IL-10 in MSCs group were increased while IFN-γ/ decreased significantly. Conclusion MSCs play an important role in regulating the inflammatory response and significantly inhibit the formation of the atherosclerosis plaque in ApoE-/-mice.