细菌视紫红质 E204Q 和 I119T/T121S/A126T突变体的构建及其功能研究

应用定点突变的方法获得了细菌视紫红质 (bacteriorhodopsin , BR) 的单突变体 BR_E204Q和三突变体 BR_{I119T/T121S/A126T}. 通过功能研究发现, BR 蛋白的单突变体 BR_E204Q的 M 态寿命为 7.10 ms ,三突变体 BR_{I119T/T121S/A126T}的 M 态寿命为 8.23 ms ,均较野生型 BR 蛋白 (6.23ms) 有所延长,三突变体表现得更为显著,其 M 态延长时间可超出野生型的 32％. 同时单突变体 BR_E204Q和三突变体 BR_{I119T/T121S/A126T}的质子泵功能也均有改变,都比野生型 BR 蛋白有所下降,其中三突变体 BR_{I119T/T121S/A126T}下降得更为明显.     

用实时荧光PCR方法鉴定转基因玉米T14/T25

本研究以实时荧光PCR技术鉴定商业化种植的转基因玉米T14/T25品系。根据转基因玉米T14/T25转入的外源基因质粒图谱,设计转基因引物和探针进行PCR和实时荧光PCR检测,建立了转基因玉米品系鉴定的实时荧光PCR方法。实验结果表明,用TaqMan探针可检测到T14/T25产生的荧光信号,而对其他玉米品系则检测不到荧光信号,为转基因产品的鉴定检测提供了新方法。Abstract: To identify genetically modified (GM) maize T14/T25 lines, a real-time fluorescent PCR (RTF PCR) assay was performed in this study. Primers and Taqman probes specific for inserted genes in the T14/T25 were used to conduct the real-time fluorenscent (RTF) PCR and PCR assays. The RTF PCR method was established to detect and identify GM maize lines. The results show that the TaqMan probe could identify T14/T25 maize used, while other GM and NO-GM maize didn’t be detected. The RTF PCR could be a new method for detecting other genetically modified organism.     

Suppression of cytotoxic T lymphocyte activity by γ/δ T cells in tumor-bearing mice

Spleen cells derived from tumor-bearing mice prove useful for the elucidation of the mechanism determining how tumor cells evade cytotoxic T lymphocytes (CTL) in tumor-bearing hosts. Our data indicate that inactive CTL or precursor CTL specific for tumor antigens are present among lymphocytes of tumor-bearing mice. However, their activity is inhibited by a soluble factor produced by other cells present in the same source. Inhibition of the cytolytic reaction was also detected in the culture supernatant of spleen cells obtained from normal mice, precultured in the presence of tumor cell culture supernatant and interleukin-2 (IL-2). Cell-depletion and cell-purification studies let us conclude that cells that produced the CTL-inhibitory factor (CTL-IF) were / T cells. The / T cells that were activated in vivo in tumor bearers were able to produce CTL-IF after isolation and in vitro culture. Maximum activation of / T cells was achieved by antigenic stimulation and by suppression of cells that interfered with the activation of / T cells. CTL-IF, which was assayed by use of CTL clones, did not show antigen specificity. Inhibition depended on a relatively heat- and acidstable, but alkali-labile molecule with a molecular mass of less than 10 kDa. The latter characteristics imply that CTL-IF does not resemble any of the known lymphokines produced by / T cells. These observations emphasize the crucial role of the / T cells in the escape of tumor cells from the attack of tumorspecific CTL.     

应用T/A策略克隆乙肝病毒pC/C及C基因

以克隆乙型肝炎病毒pC/C及C基因为例,报道了在DNA重组中,当目的基因与载体末端不匹配时可采取的一新方法.用内切酶切取的基因片段为平端时,可在含dATP的反应体系中,用Taq酶的末端转移酶活性在其3′末端加上单个碱基(dA)的突出尾;基因片段为3′凹端时,可在含4种dNTP的体系中,利用Taq酶的聚合酶活性先将其末端补平,再经末端转移酶活性在其3′末端加dA尾;末端经此修饰的基因片段可亚克隆至T载体中,再克隆于其他表达载体中.     

Association of TGF-β1 − 509 C/T, 29 C/T and 788 C/T gene polymorphisms with chronic periodontitis: A case–control study

The aim of this study was to investigate the possible association between TGF-β1 − 509 C/T (rs1800469), 29 C/T (Prol10Leu, rs1800470) and 788 C/T (Thr263Ile, rs1800472) gene polymorphisms and chronic periodontitis (CP) in a sample of Iranian population. This case–control study was conducted on 100 CP patients and 100 healthy unrelated, age-, sex-, and ethnicity-matched. Genotyping was performed by tetra amplification refractory mutation system-polymerase chain reaction (T-ARMS-PCR) technique. Our findings showed that there was a significant difference between the groups regarding TGF-β1 29 C/T (rs1800470) polymorphism (χ2 = 23.23, P < 0.0001). The CT and TT genotypes increased the risk of CP in comparison with the CC genotype (OR = 4.42, 95% CI = 2.16–9.06, P < 0.001 and OR = 5.84, 95% CI = 2.32–14.71, P < 0.001, respectively). The T allele increased the risk of CP (OR = 2.50, 95% CI = 1.66–3.74, P < 0.001) in comparison with C allele. No significant association was found among the groups regarding − 509 C/T and 788 C/T variants of TGF-β1 gene. This study shows that TGF-β1 29 C/T polymorphism, but not − 509 C/T and 788 C/T polymorphisms, may contribute to the development of CP in a sample of Iranian population. Further studies with larger sample sizes and different ethnicities are needed to validate our findings.     

Interleukin-1β-31C/T and -511T/C Polymorphisms Were Associated with Preeclampsia in Chinese Han Population

Objective

The purpose of our study is to investigate the relationship between IL-1β -31C/T (rs1143627) and -511T/C (rs16944) polymorphisms and the preeclampsia (PE), and analyze the Linkage disequilibrium (LD) and haplotype frequency of the two polymorphism loci.

Methods

Polymorphisms at -31C/T and -511T/C of IL-1β were genotyped with the method of polymerase chain reaction-restriction fragment length polymorphism (PCR- RFLP) in 232 PE and 447 control subjects. Genotype and allele frequencies between case-control groups were compared by chi-square(X²) tests. Two-point LD and haplotype frequency analyses were done with the software Haploview4.2.

Results

Significant statistical differences were found between PE and control groups regarding genotype and allele frequencies of the two polymorphisms of IL-1β (For IL-1β -31C/T: X² = 11.478, P = 0.003; For IL-1β-511T/C: X² = 9.687, P = 0.008). LD analysis revealed that the IL-1β -31C/T SNP was in high LD with the IL-1β-511C/T SNP(D′ = 0.92, r² = 0.79). Both CT and TC haplotypes showed significant differences between case and control groups. Only the plasma level of Prothrombin Time had a significantly statistical difference among TT, CT and CC groups of the preeclamptic two polymorphisms of IL-1β-31C/T and -511T/C (for IL-1β-31C/T, F = 1.644, P = 0.01; F = 1.587, P = 0.016).

Conclusion

Our results revealed IL-1β was associated with the PE in Chinese Han population. The CT haplotype may increase the risk of PE, while haplotype TC could be considered as a protective haplotype of PE.     

Signal transduction via the T cell antigen receptor in naïve and effector/memory T cells

T cells play an indispensable role in immune defense against infectious agents, but can also be pathogenic. These T cells develop in the thymus, are exported into the periphery as naïve cells and participate in immune responses. Upon recognition of antigen, they are activated and differentiate into effector and memory T cells. While effector T cells carry out the function of the immune response, memory T cells can last up to the life time of the individual, and are activated by subsequent antigenic exposure. Throughout this life cycle, the T cell uses the same receptor for antigen, the T cell Receptor, a complex multi-subunit receptor. Recognition of antigen presented by peptide/MHC complexes on antigen presenting cells unleashes signaling pathways that control T cell activation at each stage. In this review, we discuss the signals regulated by the T cell receptor in naïve and effector/memory T cells.     

Do cytotoxic T lymphocytes clear some HIV/SIV infections?

Early work on the roles of cytotoxic T lymphocytes (CTLs) in acute viral infections in animal models showed that i) the clearance of virus coincided with the increase in CTL activity rather than specific antibody levels, ii) transfer of CTLs after infection could protect from a lethal dose of virus, and iii) in primed, compared to naive, animals, CTL activity appeared 1–3 days earlier after a challenge infection. There is now a series of findings with individuals who have been exposed to HIV but are HIV-seronegative that suggest a protective role for CTLs. Usually after in vitro culture, HIV-specific CTLs have been isolated from i) infants born of infected mothers, ii) long-time partners of HIV-infected people, iii) some prostitutes in Africa, and iv). Most recently, 7/20 seronegative health care workers exposed once to HIV have been shown to possess HIV env-specific CTLs. The findings suggest that CTLs (a type I T cell response) may rapidly clear a low dose of HIV. Experiments with SIV are proposed that may provide more direct supporting data for this possibility.     

植物FLOWERING LOCUS T/TERMINAL FLOWER1基因家族的研究进展

植物FLOWERING LOCUS T/TERMINAL FLOWER1(FT/TFL1)基因家族是一个进化上高度保守的基因家族,它在植物的花发育过程中具有重要作用:其成员FT基因编码的蛋白产物是可以长距离转运的成花激素,在花形成过程中起关键作用;另一成员TFL1基因则在花序的形成和维持过程中起重要作用.本文就近年来国内外对植物FT/TFL1基因家族的结构、成员,以及各个成员在花发育转换过程中的功能等研究现状进行综述,并对该基因家族的研究前景提出展望.     

活化/抑制CD59 对T 淋巴细胞增殖的影响

目的：研究活化/抑制CD59 分子对T 细胞增殖的影响。方法：Jurkat细胞分别电转入pSUPER-siCD59 质粒及用CD59 活化 抗体刺激。激光共聚焦显微镜下观察细胞的电转情况及CD59 分子在细胞膜上的分布及表达;MTT 比色法检测细胞的增殖。 Western blot检测CD59 分子表达及T细胞活化相关蛋白ZAP70磷酸化水平。结果：激光共聚焦显微镜下可见电转染细胞表达绿 色荧光,转染效率约为40%。转染pSUPER-siCD59 质粒后CD59荧光强度强度降低,CD59 分子均匀分布于细胞膜与正常Jurkat 细胞分布一致。抗体活化后CD59 在细胞膜成簇状分布。抗体活后细胞增殖速率和磷酸化ZAP70 的蛋白表达水平均高于正常组 （P<0.05）,而细胞电转质粒后则恰恰相反。结论：CD59 通过与信号转导分子的相互作用促进T 细胞活化增殖。     

多糖调控T/B淋巴细胞免疫应答机制的研究进展

淋巴细胞是机体适应性免疫系统的重要组成,多糖对其刺激作用在生物医药领域受到广泛的关注。目前,大部分的相关研究仅限于多糖对淋巴细胞增殖及细胞因子或抗体表达水平的调控,系统的分子机制解析少见报道。综合多糖对淋巴细胞的免疫调节作用发现:活性多糖可同时刺激T/B细胞、也可选择性刺激T细胞或选择性刺激B细胞;多糖刺激T细胞免疫应答的信号通道主要为TCR/CD3→PTK→PI3-K→PKC/PLCγ→Ca2+→calcineurin→NFAT和TCR/CD3→PTK→MAPKs→AP-1;而刺激B细胞的信号通道主要包括TLR2/4→TRAF6→IKKc→NF-κB、TLR2/4→PTK→MAPKs→AP-1和IgM/CD79→PTK→MAPKs→AP-1。同时,归纳多糖刺激淋巴细胞活性的构效关系,旨在为相关领域的研究提供参考。     

γ/δ T细胞与丙型肝炎病毒、乙型肝炎病毒感染

病毒性肝炎的发病机制迄今尚未完全明确,诸多证据表明,乙型肝炎病毒(HBV)及丙型肝炎病毒(HCV)所致肝炎可能是肝脏细胞免疫防御反应病毒入侵的结果。γ/δT细胞是新近认识的一个T细胞亚群,是机体抵抗外来病原微生物入侵的重要天然免疫细胞之一。近年研究发现,肝内富含γ/δT细胞,而病毒性肝炎肝内γ/δT细胞数量显著增高。目前有关γ/δT细胞与肝炎病毒感染的研究主要集中在HCV感染领域,即γ/δT细胞通过分泌多种细胞因子抑制体内HCV的复制。目前,有关γ/δT细胞与HBV感染的报道甚为少见。慢性HBV感染体内可能导致γ/δT细胞免疫学功能异常,这可能是导致体内病毒性乙型肝炎慢性化的主要原因之一。     

Anti-CD20scFv/IgGFc/CD80/CD28/zeta转染人T淋巴细胞对原代CLL细胞的作用

目的:将已成功构建表达anti-CD20scFv/CD80/CD28/zeta转染人T淋巴细胞,体外观察该类细胞特异性清除CD20+原代慢性淋巴细胞白血病(CLL)细胞的能力,为肿瘤的过继免疫治疗提供新思路。方法:将本室成功构建的含anti-CD20scFv/IgGFc/CD80片段的PLNCX质粒,转染PA317包装细胞,挑取高滴度的包装细胞株收获逆转录病毒,用收获的病毒感染刺激分裂的人外周血T细胞,经G418筛选后与CD20+原代CLL细胞在体外共同培养,在显微镜下观察CD20+的原代CLL细胞生长状态,ELISA检测试剂盒检测T细胞分泌细胞因子的功能。结果:重组基因修饰的T细胞能在体外杀伤CD20+原代CLL细胞,而对CD20-细胞无杀伤作用;同时靶细胞为CD20+组上清液中IL-2(1301.00pg/ml)和IFN-γ(602.18pg/ml)水平与CD20-组相比明显升高。结论:嵌合锚定T细胞能够成功构建;该类T细胞在体外能特异性杀伤CD20+的原代CLL细胞。     

HTLV-1感染T细胞克隆扩增和转化在成人T细胞白血病表达分析

摘要 目的：探究人类T细胞白血病1型病毒（Human T-cell leukemia virus type，HTLV-1）感染的T细胞克隆扩增和转化在成人T细胞白血病（AdultT-cellleukemia，ATL）中的表达分析，探究HTLV-1在T淋巴细胞中发生克隆扩增和转化的机制，为ATL的临床治疗提供理论基础。方法：选择2015年2月至2018年2月于我院接受治疗的38例ATL患者为研究对象，按照其病程差异将其分为急性ATL组（20例）和慢性ALT组（18例），分别采集其血样并检测两组患者血样中HTLV-1病毒载量的差异性，对比两组患者样本中Tax蛋白和HMGB1蛋白的表达情况，并就两组患者血样中肿瘤坏死因子（tumor necrosis factor，TNF-α）、癌胚抗原（carcinoembryonic antigen，CEA）的水平进行对比。结果：（1）急性ATL组患者HTLV-1病毒载量明显高于慢性ATL组患者HTLV-1病毒载量（P<0.05）；（2）对比显示，急性ATL组患者血样中Tax蛋白和HMGB1蛋白表达量明显高于慢性ATL组患者（P<0.05）；（3）急性ATL组患者中TNF-α和CEA水平均明显高于慢性ATL组患者（P<0.05）。结论：HTLV-1感染ATL患者病程的差异会影响T淋巴细胞的克隆扩增和转化进程，分析其机制可能与HTLV-1能够调控Tax蛋白和HMGB1表达有关。     

结外NK/T细胞淋巴瘤的风险评估与治疗进展

结外NK/T细胞淋巴瘤(extranodal NK/T-cell lymphoma,ENKTCL)是非霍奇金淋巴瘤中一种少见的亚型,其发病机制包括EB病毒感染、ENKTCL相关基因异常、信号通路的异常活化、肿瘤微环境的改变,该病病程进展快,预后较差,预后模型包括Ann Arbor分期模型、国际预后指数(IPI)模型、韩国预后指数(KPI)模型、PINK-E模型、Nomogram风险指数(NRI)模型,同时临床上已发现越来越多ENKTCL的独立预后因素,这对于ENKTCL的风险评估有着积极意义。目前,ENKTCL的治疗方案包括放化疗治疗、造血干细胞移植治疗、靶向治疗。该文对ENKTCL的发病机制、预后模型、风险评估和治疗进展进行综述,以期提高ENKTCL的诊治效果。     

耗竭性T细胞在肿瘤中的作用

耗竭性T细胞(exhausted T cells)是一群效应功能减弱,持续表达抑制性受体的T细胞,在肿瘤中表现为T细胞功能缺陷状态,主要特征为一系列抑制性受体表达增加及细胞因子分泌减少。耗竭性T细胞主要通过细胞表面的抑制性分子,细胞因子和免疫调节细胞类型改变等参与肿瘤免疫负调控,从而引起肿瘤免疫逃逸。而T细胞耗竭状态并非不可逆转,应用相应单克隆抗体靶向免疫调控点可以有效逆转耗竭性T细胞,恢复机体抗肿瘤免疫反应,提高肿瘤控制率。因此,通过逆转肿瘤患者体内的耗竭性T细胞可能是肿瘤免疫治疗的新途径之一。     

频谱水对BALB/c小鼠T淋巴细胞转化的影响

目的探讨频谱水对实验小鼠细胞免疫功能的影响。方法将60只SPF级BALB/c小鼠随机分成喝泡频谱水组、喝自来水泡频谱水组、喝泡自来水组（对照组）,分别检测每组经ConA处理后T淋巴细胞转率。结果前两组处理组与对照组相比较,T淋巴细胞转化率增高,差异有显著性。结论频谱水可以提高机体的细胞免疫功能。     

Chimeric IgH-TCRα/δ translocations in T lymphocytes mediated by RAG

Translocations involving the T cell receptor alpha/delta (TCRα/δ) chain locus, which bring oncogenes in the proximity of the TCRα enhancer, are one of the hallmark features of human T cell malignancies from ataxia telangiectasia (AT) and non-AT patients. These lesions are frequently generated by the fusion of DNA breaks at the TCRα/δ locus to a disperse region centromeric of the immunoglobulin heavy chain (IgH) locus. Aberrant VDJ joining accounts for TCRα/δ associated DNA cleavage, but the molecular mechanism that leads to generation of the "oncogene partner" DNA break is unclear. Here we show that in ATM deficient primary mouse T cells, IgH/TCRα/δ fusions arise at a remarkably similar frequency as in human AT lymphocytes. Recombinase-activating gene (RAG) is responsible for both TCRα/δ as well as IgH associated breaks on chromosome 12 (Chr12), which are subject to varying degrees of chromosomal degradation. We suggest a new model for how oncogenic translocations can arise from two non-concerted physiological DSBs.     

大肠杆菌等受体tRNALeu的T7 RNA聚合酶转录

用化学方法合成编码 2个大肠杆菌tRNA^Leu(tRNA^Leu₁和tRNA^Leu₂ )的基因和T7启动子 ,分别克隆到pUC1 9载体上 ,并在纯化的T7RNA聚合酶的体外转录系统中转录出不含修饰核苷酸的tRNA^Leu.在T7转录体系中 ,亚精胺对转录有负影响 .在最适转录条件下 ,可以得到有活力的RNA转录物的量是模板DNA的 2 5 0倍左右 .在大肠杆菌亮氨酰 tRNA合成酶的催化下 ,2种经体外转录产生的未修饰等受体tRNA^Leu(tRNA^Leu₁和tRNA^Leu₂ )的亮氨酸接受能力基本相同 ,但只有从体内纯化对应的tRNA^Leu的四分之一左右 ,表明修饰核苷酸在tRNA^Leu氨酰化过程中起着较为重要但非关键的作用 .