CD4~+T、CD8~+T、CD4~+/CD8~+与慢性乙肝不同中医体质存在相关性

探讨外周血CD4~+、CD8~+T水平与慢性乙型肝炎不同中医体质的关系。选取2016年2月至2017年3月在我院治疗的慢性乙型感染患者143例,其中平和质35例、气虚质40例、阴虚质21例、湿热质20例,气郁质16例、其他11例,采用流式细胞仪检测外周血T淋巴细胞亚群。不同中医体质患者性别、年龄、病程及HBV-DNA含量比较差异无统计学意义(p0.05);平和质患者AST为342.21(142.42,513.46)U/L,明显低于其他患者(p0.05);气虚质患者AST为512.40(322.81,726.50)U/L,明显高于其他患者(p0.05);气郁质及其他体质患者ALT分别为381.64(210.41,501.72)U/L和370.43(200.41,470.63)U/L,明显高于平和质、气虚质、阴虚质和湿热质患者(p0.05);平和质和气虚质患者外周血CD4~+T细胞分别为(39.10±2.01)%和(39.10±2.01)%,明显低于阴虚质、湿热质、气郁质及其他体质患者(p0.05);气郁质及其他体质患者CD8~+T细胞分别为(25.43±1.33)%和(25.24±1.31)%,明显低于平和质、气虚质、阴虚质和湿热质患者(p0.05);阴虚质、气郁质及其他体质患者分别为(1.71±0.09)、(1.75±0.08)和(1.78±0.09),明显高于平和质、气虚质和湿热质患者(p0.05)。慢性乙肝不同中医体质与CD4~+T、CD8~+T和以及肝功能有密切关系。关键词     

紫外线照射下小鼠T细胞CD4和CD8的表达

紫外线对机体健康的影响主要有物理性损伤 ,如引起皮肤表面的红肿 ,疼痛 ,出现水泡 ,产生皱褶 ,并出现色素沉着 ,皮肤老化等现象。严重者由于紫外线对机体的光毒性作用 ,皮肤内的各种色素集团在吸收光线的同时产生大量的氧自由基 ,进而造成ＤＮＡ分子的损伤 ,引起基因突变、癌化 ,直至细胞死亡。近年来有研究报道 ,通过紫外线照射 ,抑制机体的细胞免疫机能 ,降低接触性迟发型超敏反应 ,甚至由于抑制Ｔ细胞而出现对特异性半抗原无免疫反应状态 ,但同时也使机体对细菌、寄生虫等的侵袭易感。为进一步探讨紫外线照射对机体免疫防御机能的影响 ,…     

鲤主要免疫器官CD4L、CD8α和CD8β表达细胞的分布特征

自1975 年在硬骨鱼类中发现T 细胞存在的证据1以来, 单克隆抗体技术、免疫组化和原位杂交等技术的应用, 使鱼类T 细胞及其亚群和功能的研究成为可能。从20 世纪80 年代起, 人们开始尝试通过各种方法例如用胸腺细胞、多聚甲醛固定的胸腺细胞(DLT15)、胸腺细胞膜(WCL9)、肠白细胞膜(WCL38)免疫小鼠进而制备抗鱼类T细胞的单克隆抗体。       

Selective support of a mouse thymus epithelial cell line （MTEC1） to the viability and proliferation of CD4＋CD8—,CD4^—CD8^—,and CD4^＋CD8^＋thymocytes in vitro

The MTEC1 cell line,established in our laboratory,is a normal epithelial cell line derived from thymus medulla of Balb/c mice and these cells constituteively produce multiple cytokines.The selection of thymic microenvironment on developing T cells was investigated in an in vitro system.Unseparated fresh thymocytes from Balb/c mice were cocultured with MTEC1 cells or/and MTEC1-SN,then,the viability,proliferation and phenotypes of cultured thymocytes were assessed.Without any exogenous stimulus,both MTEC1 cells and MTEC1-SN were able to maintain the viability of thymocytes,while only the MTEC1 cells,not the MTEC1-SN,could directly activate thymocytes to exhibit moderate proliferation,indicating that the proliferative signal is delivered through cell surface interatcions of MTEC1 cells and thymocytes.Phenotype analysis on FACS of viable thymocytes after coculture revealed that MTEC1 cells preferentially activate the subsets of CD4^ CD8^-,CD4^ CD^8 and CD^4- CD^8- thymocytes;whereas MTEC1-SN preferentially maintained the viability of CD4^ CD^8- and CD4^-CD8^ thymocyte subsets.For the Con A-activated thymocytes.both MTEC1 cells and MTEC1-SN provided accessory signal(s) to significantly increase the number of viable cells and to markedly enhance the proliferation of thymocytes with virtually equal potency,phenotyped as CD4^ CD8^-,CD4^-CD8^ ,and CD^4-CD8^-subests,In summary,MTEC1 cells displayed Selection of thymic epithelial cells on thymocyte subsets. selective support to the different thymocyte subsets,and the selectivity is dependent on the status of thymocytes.     

Distinct and overlapping effector functions of expanded human CD4+, CD8α+ and CD4-CD8α- invariant natural killer T cells

CD1d-restricted invariant natural killer T (iNKT) cells have diverse immune stimulatory/regulatory activities through their ability to release cytokines and to kill or transactivate other cells. Activation of iNKT cells can protect against multiple diseases in mice but clinical trials in humans have had limited impact. Clinical studies to date have targeted polyclonal mixtures of iNKT cells and we proposed that their subset compositions will influence therapeutic outcomes. We sorted and expanded iNKT cells from healthy donors and compared the phenotypes, cytotoxic activities and cytokine profiles of the CD4(+), CD8α(+) and CD4(-)CD8α(-) double-negative (DN) subsets. CD4(+) iNKT cells expanded more readily than CD8α(+) and DN iNKT cells upon mitogen stimulation. CD8α(+) and DN iNKT cells most frequently expressed CD56, CD161 and NKG2D and most potently killed CD1d(+) cell lines and primary leukemia cells. All iNKT subsets released Th1 (IFN-γ and TNF-α) and Th2 (IL-4, IL-5 and IL-13) cytokines. Relative amounts followed a CD8α>DN>CD4 pattern for Th1 and CD4>DN>CD8α for Th2. All iNKT subsets could simultaneously produce IFN-γ and IL-4, but single-positivity for IFN-γ or IL-4 was strikingly rare in CD4(+) and CD8α(+) fractions, respectively. Only CD4(+) iNKT cells produced IL-9 and IL-10; DN cells released IL-17; and none produced IL-22. All iNKT subsets upregulated CD40L upon glycolipid stimulation and induced IL-10 and IL-12 secretion by dendritic cells. Thus, subset composition of iNKT cells is a major determinant of function. Use of enriched CD8α(+), DN or CD4(+) iNKT cells may optimally harness the immunoregulatory properties of iNKT cells for treatment of disease.     

Identification of CD3ε, CD4, CD8β splice variants of Atlantic salmon

In vertebrates, CD3 complex and CD4 and CD8 co-receptors are essential for signal transduction during T cell activation. In the present study, we report the mRNA spliced variants of the Atlantic salmon CD3ε, CD4 and CD8β and the effect of pathogen encounter on the expression of these variants. CD3ε is alternatively spliced in thymus, head kidney, spleen and gills to give rise to the complete mRNA sequence and to an alternative product that lacks the transmembrane exon. CD4 is also alternatively spliced in the thymus, head kidney, spleen and gills to form two variants, although the alternative product is barely detectable. The alternative product lacks the exon 1B encoding the D1 domain, which is essential for binding to MHC class II proteins. Two amplicons were also found for the CD8β gene; sequencing analysis revealed that the main PCR product corresponds to the previously reported CD8β sequence, whereas the variant sequence encodes a potential protein that lacks the Ig-like domain. The expression of CD3, CD4, CD8β genes also analyzed in head kidney of LPS-treated and IPNV infected salmon and different patterns of expression were observed. The presence and balance of the different variants of T cell co-receptors could be related to the ability of fish to induce a particular type of immune response, as well as, the ability of the pathogen to modify the fish immune response.     

记忆性CD8细胞产生、维持及CD4细胞的辅助作用

记忆性T淋巴细胞的形成及其在体内的长期维持,是一个复杂的多层次调控过程,CD4细胞及相关的细胞因子通过间接和直接作用,对CD8记忆细胞的形成起到重要的促进作用。CD8记忆细胞需要不同信号的刺激以保证其在体内的长期维持,是一个动态平衡的过程。     

In Vivo Dynamical Interactions between CD4 Tregs,CD8 Tregs and CD4+CD25? Cells in Mice

Background

Regulatory T cells (Tregs) were shown to be central in maintaining immunological homeostasis and preventing the development of autoimmune diseases. Several subsets of Tregs have been identified to date; however, the dynamics of the interactions between these subsets, and their implications on their regulatory functions are yet to be elucidated.

Methodology/Principal Findings

We employed a combination of mathematical modeling and frequent in vivo measurements of several T cell subsets. Healthy BALB/c mice received a single injection of either hCDR1 - a tolerogenic peptide previously shown to induce Tregs, a control peptide or vehicle alone, and were monitored for 16 days. During this period, splenocytes from the treated mice were analyzed for the levels of CD4, CD25, CD8, CD28 and Foxp3. The collected data were then fitted to mathematical models, in order to test competing hypotheses regarding the interactions between the followed T cell subsets. In all 3 treatment groups, a significant, lasting, non-random perturbation of the immune system could be observed. Our analysis predicted the emergence of functional CD4 Tregs based on inverse oscillations of the latter and CD4⁺CD25⁻ cells. Furthermore, CD4 Tregs seemed to require a sufficiently high level of CD8 Tregs in order to become functional, while conversion was unlikely to be their major source. Our results indicated in addition that Foxp3 is not a sufficient marker for regulatory activity.

Conclusions/Significance

In this work, we unraveled the dynamics of the interplay between CD4, CD8 Tregs and effector T cells, using, for the first time, a mathematical-mechanistic perspective in the analysis of Treg kinetics. Furthermore, the results obtained from this interdisciplinary approach supported the notion that CD4 Tregs need to interact with CD8 Tregs in order to become functional. Finally, we generated predictions regarding the time-dependent function of Tregs, which can be further tested empirically in future work.     

TCRαβ~ CD4~ CD8~-胸腺髓质细胞的表型分析

本实验综合分析了CD4~ CD8~-胸腺髓质细胞多种表面分子的表达情况。通过抗体加补体的2次杀伤和panning方法,分离出CD4~ CD8~-胸腺髓质细胞,进行直接或间接荧光抗体染色,利用流式细胞仪分析细胞表型。发现CD4~ CD8~-胸腺细胞均为TCRαβ阳性,但CD69,HSA,Qa-2,3G11,6C10分子呈现异质性表达。利用多个表面分子组合进行双染FACS分析,推测CD4SP胸腺细胞由不成熟到发育成熟,迁出胸腺,可分为7个阶段:(1)3G11~-6C10~ CD69~ HSA~(hi),(2)3G11~ 6C10~ CD69~ HSA~(hi),(3)3G11~ 6C10~-CD69~ HSA~(int),(4)3G11~ 6C10~-CD69~-HSA~(int)Qa-2~-,(5)3G11~ HSA~(lo/-)Qa-2~(lo),4阶段还可进一步分化为(6) 3G11~-HSA~(lo)Qa-2~-,(7) 3G11~-HSA~(lo/-)Qa-2~(hi)。Qa-2~ 的5,7两阶段细胞已达到最终成熟,并可迁出胸腺。     

应用流式细胞术分析林麝外周血 CD4+、CD8+ T淋巴细胞

通过对圈养林麝(Moschusberezovskii)外周血淋巴细胞CD4~+、CD8~+亚群的检测,探讨林麝细胞免疫功能状态,并探索应用流式细胞仪分析其淋巴细胞亚群的方法,为研究林麝重大疾病的病理机制及诊断方法提供科学依据。本研究选取健康林麝和患呼吸道疾病林麝各5头,以双色流式细胞术检测其外周血淋巴细胞CD4~+、CD8~+亚群的含量,并进行比较。结果显示,羊源CD4、CD8的流式荧光抗体能够标记林麝细胞并有效检测;患病林麝与健康林麝相比,外周血CD4~+细胞含量无差异(P 0.05),CD8~+细胞含量则显著降低(P 0.01),CD4~+/CD8~+比值显著增高(P 0.01)。结果表明,患呼吸系统炎性疾病的林麝其外周血淋巴细胞CD8~+亚群变化显著,检测淋巴细胞亚群对林麝疾病的诊断有重要意义。     

不同电镜分型女性生殖道尖锐湿疣的CD4+、CD8+的表达

目的:探讨不同电镜分型的女性生殖道尖锐湿疣(CA)的免疫应答状态的异同.方法:将随机抽取的50例女性生殖道尖锐湿疣的活栓组织按照扫描电镜和透射电镜下形态学特征分为尖锐型湿疣、结节型湿疣和内生型湿疣三组.以免疫组织化学方法(IHC)研究CD4+T细胞、CD8+T细胞、CD4+/CD8+比值于不同电镜分型CA中的表达.结果:结节型湿疣的CD4+T细胞数及CD4+/CD8+比值均显著低于尖锐型湿疣,内生型湿疣介于二者之间.结论:CD4+/CD8+比值在不同类型CA中的表达结果有统计学差异,结节型湿疣免疫应答状态异常,预示三种电镜分型的尖锐湿疣转归不同.CD4+/CD8+比值可作为判断预后的指标.     

Human CD8⁺ and CD4⁺ T cell memory to lymphocytic choriomeningitis virus infection

Although cellular immunity to acute lymphocytic choriomeningitis virus (LCMV) infection has been well characterized in experimental studies in mice, the T cell response to this virus in humans is incompletely understood. Thus, we analyzed the breadths, magnitudes, and differentiation phenotypes of memory LCMV-specific CD8(+) and CD4(+) T cells in three human donors displaying a variety of disease outcomes after accidental needle stick injury or exposure to LCMV. Although only a small cohort of donors was analyzed at a single time point postinfection, several interesting observations were made. First, we were able to detect LCMV-specific CD8(+) and CD4(+) T cell responses directly ex vivo at 4 to 8 years after exposure, demonstrating the longevity of T cell memory in humans. Second, unlike in murine models of LCMV infection, we found that the breadths of memory CD8(+) and CD4(+) T cell responses were not significantly different from one another. Third, it seemed that the overall CD8(+) T cell response was augmented with increasing severity of disease, while the LCMV-specific CD4(+) T cell response magnitude was highly variable between the three different donors. Next, we found that LCMV-specific CD8(+) T cells in the three donors analyzed seemed to undergo an effector memory differentiation program distinct from that of CD4(+) T cells. Finally, the levels of expression of memory, costimulatory, and inhibitory receptors on CD8(+) and CD4(+) T cell subsets, in some instances, correlated with disease outcome. These data demonstrate for the first time LCMV-specific CD8(+) and CD4(+) T cells in infected humans and begin to provide new insights into memory T cell responses following an acute virus infection.     

Age-associated changes in interferon-γ and interleukin-4 secretion by purified human CD4+ and CD8+ T cells

Aging is associated with a decline in immune function. Interferon-gamma (IFN-gamma) and interleukin-4 (IL-4), two important immune deviation-related cytokines, are mainly produced by type 1 and type 2 T cells, respectively. To investigate the age-associated changes in the secretion of these two cytokines, 20 elderly and 20 young subjects fulfilling the SENIEUR protocol were enrolled. The ratios of CD4+ to CD8+ T cells were not different between the two age groups. The CD4+ and CD8+ T cells were purified by a magnetic cell sorting system, and then activated by concurrent anti-CD3 and anti-CD28 stimulation. The released cytokines were determined by ELISA. Both the CD4+ and the CD8+ T cells of the elderly individuals secreted a significantly larger amount of IFN-gamma after activation. Profound IL-4 production by CD8+ T cells was observed in the older subjects compared with that of the young subjects. These data suggested that age-associated decrease in immunity may be related to an imbalance in the secretion of immune deviation cytokines. The number of IL-4-secreting CD8+ T cells (T cytotoxic 2) rose significantly in the older individuals. Our design also provided a useful way to differentiate the T cell subsets secreting the same cytokine, such as IFN-gamma-producing T helper 1 and T cytotoxic 1 cells.     

E.tenella感染鸡CD4+、CD8+T细胞的动态变化研究

用免疫组化ABC法检测了柔嫩艾美耳球虫(E.tenella)感染雏鸡后各免疫器官和盲肠局部的T淋巴细胞亚群CD4 淋巴细胞和CD8 T淋巴细胞数的动态变化。结果表明:(1)雏鸡初次感染E.tenella后,免疫器官盲肠扁桃体、脾脏、胸腺和盲肠黏膜中的CD4 T淋巴细胞均于第2天开始增殖,第6天~8天达到峰值;二次感染后第2天有短暂的下降,第5天开始缓慢回升,第8天二次达到峰值,但第二个峰值比第一个峰值低,说明CD4 T淋巴细胞积极参与启动免疫应答和抵抗初次感染。(2)雏鸡初次感染E.tenella后,免疫器官法氏囊、盲肠扁桃体、脾脏、胸腺和盲肠黏膜中的CD8 T淋巴细胞都于第2天开始增殖,第8天达到峰值;二次感染后立即回升,第5天达到峰值,然后缓慢下降,且第二个峰值比第一个峰值高,表明CD8 T淋巴细胞是抵抗再感染的主力。