实时荧光定量PCR检测人肿瘤细胞NKG2D配体基因表达

目的：建立人肿瘤细胞NKG2D配体基因（MICA、MICB、ULBP1、ULBP2、ULBP3）表达的实时荧光定量PCR（real-time fluorescence quantitativePCR）检测方法。方法：根据NCBI基因库中NKG2D配体基因序列,设计合成引物。用Trizo1法从培养的肿瘤细胞（BEC-7402、HeLa、MDA-MB-435、XWLC-05）中提取总RNA,逆转录成eDNA,建立实时荧光定量PCR检测NKG2D配体基因表达的方法,并检测NKG2D配体在肿瘤细胞株中的表达。结果：经过琼脂糖凝胶电泳、熔解曲线和标准曲线分析,用所设计的引物和SYBR GreenI能够特异扩增和定量检测NKG2D配体基因的表达。该方法成功检测4种肿瘤细胞NKG2D配体基因的表达。结论：建立了人NKG2D配体基因表达的实时荧光定量PCR检测方法,为进一步研究人NKG2D配体在肿瘤免疫中的作用提供了有效手段。     

NKG2D免疫受体及其配体的作用

受到感染或损伤的细胞通过中间受体将信号传导至机体的免疫系统,NKG2D即是这样一种典型的具有较高免疫原性的免疫受体,它的主要作用是传导受损伤细胞产生的信号,诱导机体产生免疫应答。该文总结了近期关于NKG2D和其配体的多样性,以及NKG2D和其配体在信号传导,刺激免疫细胞产生,肿瘤细胞的监督和疾病预防方面的新发现。     

NKG2D及其配体在肿瘤免疫中的研究进展

活化性受体NKG2D（natural-killer group 2,member D）及其配体在NK、γδ＋T和CD8＋T细胞介导的肿瘤免疫应答中扮演了重要角色。深入理解NKG2D及其配体在肿瘤免疫中的作用有助于临床预防和治疗肿瘤。该文阐述了NKG2D的分子结构特性、表达调控及其配体的分类和表达调控;主要介绍了NKG2D及其配体在肿瘤免疫中的作用;最后分析了NKG2D免疫途径中存在的问题和治疗应用前景。     

拟南芥CHS 基因表达的实时荧光定量PCR 检测

在简要介绍实时荧光定量PCR反应和定量原理的基础上, 采用TaqMan荧光定量PCR技术, 研究了UV-B辐射对拟南芥(Arabidopsis thaliana)CHS(查耳酮合成酶基因)表达的诱导, 获得了与传统Northern杂交一致的结果。实时荧光定量PCR用于基因表达的定量检测, 具有特异性强、自动化程度高、高效快捷, 避免使用放射性同位素, 能同时对多个样品中的起始模板进行准确定量等特点, 因此该方法已逐渐被广泛用于基因表达的定量分析。     

拟南芥CHS基因表达的实时荧光定量PCR检测

在简要介绍实时荧光定量PCR反应和定量原理的基础上,采用TaqMan荧光定量PCR技术,研究了UV-B辐射对拟南芥(Arabidopsis thaliana)CHS(查耳酮合成酶基因)表达的诱导,获得了与传统Northern杂交一致的结果.实时荧光定量PCR用于基因表达的定量检测,具有特异性强、自动化程度高、高效快捷,避免使用放射性同位素,能同时对多个样品中的起始模板进行准确定量等特点,因此该方法已逐渐被广泛用于基因表达的定量分析.     

实时荧光定量PCR技术综述

实时荧光定量PCR技术是在PCR技术基础上发展起来的一种高度灵敏的核酸定量技术。与传统PCR相比,实时定量PCR能够更加快速、灵敏,并有效地对核酸进行定量检测。     

实时荧光定量PCR技术及其应用

实时荧光定量PCR技术是一种多色荧光检测核酸定量技术,该简要介绍实时荧光定量PCR技术的原理及其应用。     

实时荧光定量PCR的数据分析方法

实时荧光定量PCR是目前检测目的核酸拷贝数及分析靶基因在mRNA表达水平相对变化的主流技术。研究表明,分析结果的准确性依赖于数据分析方法的可靠性。我们简要综述实时荧光定量PCR的数据分析方法。     

实时荧光定量PCR的应用和进展

实时荧光定量PCR技术通过检测PCR产物中荧光讯号强度来达到定量的目的,该技术不仅实现了PCR从定性到定量的飞跃,而且与常规PCR相比,它具有特异性更强、有效解决PCR污染问题、自动化程度高等特点,目前已在动植物基因工程,微生物和医学领域中得到广泛应用。本文对实时荧光定量PCR技术的原理、优缺点及近年来新兴起的荧光探针的原理、优缺点进行了评述,重点及创新点是对实时荧光定量PCR技术在动植物基因工程,微生物和医学领域的应用进行了比较全面的综述,并对实时荧光定量PCR技术的普及应用及在基因诊断领域的前景做了进一步的展望。     

实时荧光定量PCR方法快速检测转基因大豆

针对转基因大豆中普遍含有的35S启动子进行引物设计,以双链DNA染料SYBR GreenⅠ为荧光标记物,利用实时荧光定量PCR方法对大豆样品进行检测。该法检测转基因大豆的检测低限为0.005 nmol/L的35S启动子,线性范围达3个数量级,可快速区分转基因大豆和非转基因大豆,具有快速、简便、灵敏、安全、高通量、低成本等优点,可推广用于转基因植物产品的快速定量检测。     

JEV-DNA实时荧光定量标准品的构建

利用TaqMan荧光定量PCR技术,建立JEV-DNA定量标准品的制备方法。通过处理JEV减毒活疫苗提取病毒RNA,进行RT-PCR扩增目的片段,与T载体连接,转化感受态细胞,T-A克隆,测序鉴定后定量。获得预期的重组质粒,建立的标准曲线有较大的线性范围。此法制备的重组质粒标准品可用于对病毒载量进行测定。     

实时荧光定量PCR法检测转基因小鼠拷贝数

目的利用实时荧光定量PCR法鉴定转基因小鼠外源基因插入拷贝数。方法以TG-CARK转基因首见鼠为研究对象,选取小鼠的高度保守基因Fabpi为内参,利用绝对定量的实时荧光PCR法鉴定转基因小鼠拷贝数,并与传统的Southern blot方法的定量结果进行比较。结果实时定量PCR鉴定的转基因拷贝数与Southernblot法完全一致,三只TG-CARK首见小鼠的拷贝数分别为1,7,45。结论实时定量PCR技术具有高准确性、高稳定性、高通量和低成本的优点,是比传统杂交技术更好的鉴定小鼠转基因拷贝数的方法。     

ULBP4 is a novel ligand for human NKG2D

The ULBPs are a family of MHC class I-related molecules. We have previously shown that ULBPs 1, 2, and 3 are functional ligands of the NKG2D/DAP10 receptor complex on human natural killer (NK) cells. Here, we describe a new member of the ULBP family, ULBP4, which contains predicted transmembrane and cytoplasmic domains, unlike the other ULBPs, which are GPI-linked proteins. Transduction of ULBP4 into EL4 cells confers the ability to bind recombinant NKG2D and mediates increased cytotoxic activity by human NK cells, consistent with the role of ULBPs as ligands for the NKG2D/DAP10 activating receptors. Tissue expression of ULBP4 differs from other members of the family, in that it is expressed predominantly in the skin.     

人博卡病毒TaqMan探针实时定量PCR检测方法的建立及初步应用

目的:建立人博卡病毒(HBoV)核酸特异、快速、敏感的TaqMan探针实时定量PCR检测方法,并对临床样本进行检测。方法:比对编码HBoV非结构蛋白NP-1的基因序列,选取其保守片段设计引物和探针,建立实时荧光定量PCR检测方法,并与传统PCR方法进行比较,然后分别对两者的灵敏性、特异性、稳定性及临床样本检验的适用性等进行评价。结果:所建立的实时定量PCR检测方法可用于HBoV的特异性检测;相对于传统PCR所达到的250拷贝/反应的检测灵敏度,实时定量PCR的检测灵敏度可高达10拷贝/反应,检测范围为109～101拷贝/反应,且具有良好的特异性和重复性;初步用于76份临床呼吸道标本检测,检出阳性5例,高于普通PCR方法(3/76)。结论:建立了HBoV TaqMan探针实时定量PCR检测方法,并可用于临床鼻咽拭子样本的检测,为开展HBoV流行病学监测及早期临床诊断提供了技术手段。     

茶树实时荧光定量PCR分析中内参基因的选择

选择合适的内参基因是提高实时荧光定量PCR分析（qRT-PCR）准确性的先决条件。该文以茶树（Camellia sinensis）芽、叶、幼根、嫩茎、花瓣、种子和愈伤组织为材料,应用实时荧光定量PCR技术,分析了18S rRNA、GAPDH、β-actin和α-tubulin4个常用内参基因在茶树不同器官组织中的表达情况。经GeNorm和NormFinder软件分析发现,当利用荧光定量PCR分析比较茶树不同器官组织中的基因表达差异时,可选择β-actin作为校正内参基因;而比较不同成熟度的叶片和愈伤组织时,可以选择GAPDH作为校正内参基因。     

NKG2D discriminates diverse ligands through selectively mechano‐regulated ligand conformational changes

Stimulatory immune receptor NKG2D binds diverse ligands to elicit differential anti‐tumor and anti‐virus immune responses. Two conflicting degeneracy recognition models based on static crystal structures and in‐solution binding affinities have been considered for almost two decades. Whether and how NKG2D recognizes and discriminates diverse ligands still remain unclear. Using live‐cell‐based single‐molecule biomechanical assay, we characterized the in situ binding kinetics of NKG2D interacting with different ligands in the absence or presence of mechanical force. We found that mechanical force application selectively prolonged NKG2D interaction lifetimes with the ligands MICA and MICB, but not with ULBPs, and that force‐strengthened binding is much more pronounced for MICA than for other ligands. We also integrated steered molecular dynamics simulations and mutagenesis to reveal force‐induced rotational conformational changes of MICA, involving formation of additional hydrogen bonds on its binding interface with NKG2D, impeding MICA dissociation under force. We further provided a kinetic triggering model to reveal that force‐dependent affinity determines NKG2D ligand discrimination and its downstream NK cell activation. Together, our results demonstrate that NKG2D has a discrimination power to recognize different ligands, which depends on selective mechanical force‐induced ligand conformational changes.     

Clinical significance of the NKG2D ligands,MICA/B and ULBP2 in ovarian cancer: high expression of ULBP2 is an indicator of poor prognosis

Objective  To investigate the clinical significance of the expression of the NKG2D ligands MICA/B and ULBP2 in ovarian cancer. Methods  Eighty-two ovarian cancer patients and six patients without ovarian cancer from Department of Obstetrics and Gynecology of Kyoto University Hospital were enrolled in this study between 1993 and 2003. Expression of MICA/B, ULBP2, and CD57 in ovarian cancer tissue and normal ovary tissue was evaluated by immunohistochemical staining, and the relationship of these results to relevant clinical patient data was analyzed. Expression of MICs, ULBP2, and HLA-class I molecules in 33 ovarian cancer cell lines and two normal ovarian epithelial cell lines, as well as levels of soluble MICs and ULBP2 in the culture supernatants, were measured. Results  Expression of MICA/B and ULBP2 was detected in 97.6 and 82.9% of ovarian cancer cells, respectively, whereas neither was expressed on normal ovarian epithelium. The expression of MICA/B in ovarian cancer was highly correlated with that of ULBP2. Strong expression of ULBP2 in ovarian cancer cells was correlated with less intraepithelial infiltration of T cells and bad prognoses for patients, suggesting that ULBP2 expression is a prognostic indicator in ovarian cancer. The expression of NKG2D ligands did not correlate with the levels of the soluble forms of the ligands. Conclusions  High expression of ULBP2 is an indicator of poor prognosis in ovarian cancer and may relate to T cell dysfunction in the tumor microenvironment. Electronic supplementary material  The online version of this article (doi:) contains supplementary material, which is available to authorized users. This work was supported by grants from Grant-in-Aid for Scientific Research (19390426, 19591932, 18209052 and 19659421) from the Ministry of Education, Science, Sports, Culture and Technology of Japan.     

16S rDNA用作荧光定量PCR靶基因快速检测铜绿假单胞菌

对20余种细菌16SrDNAs进行多序列比对与进化树分析,设计铜绿假单胞菌(Pseudomonasaeruginosa,PA)荧光定量PCR(fluorescencequantitativePCR,FQ-PCR)特异性引物。提取PA基因组DNA,以特异性引物扩增16SrDNA靶片段,并构建重组质粒pMDT-Pfr。将梯度稀释的pMDT-Pfr质粒作为模板,用于建立定量标准曲线。以SYBRGreenI荧光染料建立20μL反应体系,对不同浓度的PADNA样品进行FQ-PCR检测。同时,以金黄色葡萄球菌、伤寒杆菌、福氏志贺菌、变形杆菌、表皮葡萄球菌、大肠杆菌和结核杆菌的基因组DNA作阴性对照,验证FQ-PCR方法检测PA的特异性。结果显示,设计的FQ-PCR引物的靶向序列,仅对PA16SrDNA有高度同源性;FQ-PCR方法检测PA,其灵敏度达3.6pg/μL的基因组DNA或(2.1×103±3.1×102)拷贝/μL的16SrDNA基因,并且具有很强的特异性;从细菌DNA提取到FQ-PCR检测,可在2h左右完成PA鉴定。较传统的培养鉴定法而言,以16SrDNA作为FQ-PCR靶基因快速检测PA,具有很好的研究价值与应用前景。