大鼠尿激酶SYBR Green Ⅰ real time RT—PCR引物的设计

设计用于SYBR Green Ⅰ法实时定量逆转录多聚酶链反应（QRT—PCR）检测大鼠尿激酶型纤溶酶原激活因子（uPA）mRNA的引物。从基因库获取靶基因及相关序列,充分收集和分析相关生物信息学数据,应用Oligo 6．22设计出一对长度为21bp的引物,其GC含量为52．4％;上下游引物3’最稳定二聚体和及发夹结构的能量分别为-1．5、-0．40kcal／mol和-3．5、-0．90kcal／mol,引物间最稳定二聚体为-3．1kcal／mol。5’端和中间AG值较高,高于3’端AG;引发效率分别455和403。实验证明,该引物能够高效、特异地实现对靶序列的检测,适用于SYBR GreenⅠ法实时定量检测（uPA）mRNA。     

四步法消除SYBR GreenⅠ实时定量RT-PCR中引物二聚体的影响

为建立一种新的SYBRgreenⅠ实时定量RT PCR方法 ,使之能够有效消除引物二聚体 (PDs)对实时定量结果的影响 .对RT PCR特异性扩增产物和PDs分别进行了凝胶电泳检测和熔解曲线分析 .依据PDs和扩增产物的熔解温度 (Tm)特点 ,在通用的三步法的延伸步骤之后 ,增加一个短暂的 (5s)恒温和荧光检测步骤 ,使这个步骤的温度高于PDs的Tm,但低于扩增产物的Tm,简称该法为四步法 .PDs的Tm 通常高于 72℃ ,但低于扩增产物的Tm .将四步法第四步的温度设置在高于PDs的Tm ,但低于扩增产物的Tm 时 ,四步法能够有效地消除PDs的影响 .对三步法和四步法SYBRgreenⅠ实时定量RT PCR进行了比较 ,发现三步法根本不能用于RNA的实时定量 ,而四步法能够实现包括低丰度RNA在内的RNA的定量 .选择Tm 值尽可能小的引物 ,使PDs与扩增产物Tm 值之间有足够的差距 ,将更有利于四步法的应用 ,并可成功地用于低丰度RNA的准确定量     

PCR引物设计及软件使用技巧

介绍了使用软件设计PCR引物的技巧。在PCR引物设计原则的基础上 ,详细介绍了两种常用引物设计软件的基本使用方法 ,并对其各自的优缺点进行了比较。一般性引物自动搜索可采用“PremierPrimer 5”软件 ,而引物的评价分析则可采用“Oli go6”软件。     

MutPrimerDesign:用于人类基因编码区域突变位点的引物设计程序

位于基因编码区的DNA突变与基因的功能密切相关。在已知人类基因编码区的突变位点时,如何在基因组上设计引物验证该突变是一个重要的问题。本文利用Python语言开发了引物设计程序MutPrimerDesign。MutPrimerDesign通过解析人类基因组序列数据库以及基因注释信息,转换基因编码区坐标为基因组坐标,并调用Primer3的python程序包接口,可批量自动化完成基因突变位点的引物及探针序列设计。MutPrimerDesign使用简便,可识别多种数据库的基因名称,并能够修改引物常规参数,实现引物的快速调整。     

SYBR Green I荧光RT-PCR检测犬瘟热方法的建立和应用

根据GenBank发表的犬瘟热病毒（CDV）的F基因序列,经过分析在F片段的保守区域内设计引物,建立了SYBR Green I荧光RT-PCR检测CDV的方法,并通过对厦门市宠物医院收集的临床发病和疑似发病的犬病料（包括眼分泌物、鼻拭子、唾液、血液、尿液等）的检测,结果表明,本研究建立的快速检测CDV的SYBR Green I荧光RT-PCR方法具有特异性强、灵敏度高、操作简便等优点,值得推广应用。     

SYBR Green I荧光RT-PCR法检测贝类中的诺如病毒

针对诺如病毒II型的保守区域设计引物,建立了SYBR Green I实时荧光RT-PCR检测诺如病毒II型的反应体系。此方法的病毒检测下限达到102拷贝,标准曲线的线形范围为102~106拷贝,相关系数为0.9952,斜率为?2.982,截距为35.84。对诺如病毒II型检测特异,与轮状病毒、腺病毒、甲肝病毒、星状病毒无交叉反应。针对质粒标准品检测的批内试验变异系数 (CV) 为0.95％~1.69％ (n=5),批间试验CV为0.87％~1.24％ (n=3)。运用此方法随机检测30份贝类水产品,检测出2份阳性样品。结果表明,SYBR Green I荧光RT-PCR检测诺如病毒II型的方法灵敏、特异、重复性好,可应用于贝类水产品的快速检测。     

用于聚合酶链式反应(PCR)引物设计的计算机程序

 本文报道了两个用于PCR引物设计的计算机程序PCRDESN和PCRDESNA。PCRDESN程序主要从以下4个方面评价用户自己设计的一对引物的质量:(1)引物内的碱基反向重复或发夹结构,(2)两个引物之间的碱基互补配对,(3)两个引物之间的同源性,(4)引物的碱基组成及特点和T_m值计算。通过用多例文献发表的及本院有关实验室提供的引物对序列的验证,确定了程序的运算参数,证明该程序能较好地检验引物对的质量和解释某些PCR实验失败的原因。PCRDESNA程序采用逐级优化的方法和比PCRDESN所选用的更严紧的引物选择参数对用户提供的核酸序列进行快速检索,以确定所有可能的和合适的引物对。     

MethyScan：一种甲基化特异性PCR引物设计及评估工具

DNA甲基化是重要的表观遗传现象,对基因表达发挥重要调控功能.大量研究表明,基因DNA甲基化是重要的临床诊断生物标志物.在临床上,实施快速、准确的DNA甲基化状态检测是诊断应用的前提和关键.甲基化特异性PCR(methylation specific PCR,MSP)通过将两种引物与甲基化、非甲基化模板各自特异性结合和扩增,实现基因甲基化状态的区分,是切实可行、简单便捷的临床诊断实验技术.但是,不同于常规PCR,MSP主要存在如何强化引物-甲基化/非甲基化模板特异性结合、降低引物序列Tm值差异、去除假阳性扩增及提高敏感性等四大难点.尽管大多数MSP引物设计软件对上述难题都提出了各自解决办法,但在引物设计影响因素考虑、设计与评估并行处理及特异性扩增预测等方面仍然存在较大缺陷.为此,本研究通过对MethPrimer、MSPPrimer、MethBlast、BiSearch等现有MSP引物设计软件原理的深入探究,以及对Bowtie、SAMtools和BEDTools等工具的有效综合整合,基于图形库Matplotlib和第三方Python功能库BioPython与Primer3-py实现了具有系列优点的甲基化特异性PCR引物设计与评估可视化工具MethyScan.它具有引物设计、基因组索引、引物评估等三大完整功能模块,不仅可快速进行MSP引物设计,实现巢式(Nested)引物适配,还可基于4种基因组碱基转换模板分析引物结合信息,图形化展示非特异性扩增与目的片段差异,从而综合评估引物特异性-非特异性扩增.同时,对食管癌、结直肠癌等多种恶性肿瘤中6个潜在生物标志物TFPI-2、NDRG4、CDKN2A、CD44、CASP8和SDHD的甲基化引物设计对比结果表明,MethyScan不仅可获得更多CpG位点的检测引物,而且所获得MSP引物位置与其他软件结果相同或相近,且引物间Tm值差值更小.总之,作为首个图形化展示特异性-非特异性扩增差异MSP引物设计工具,MethyScan可有效提高甲基化引物设计准确性,为临床DNA甲基化检测项目开展、检测试验实施及诊断试剂盒研发提供有力支撑.MethyScan工具下载地址:https://github.com/bioinfo-ibms-pumc/MethyScan.     

原核细胞mRNA差异显示技术的引物设计

由于原核细胞mRNA3'端不存在ploy(A)结构,因而原核细胞DDRT-PCR引物设计不同于真核细胞。尽管不能根据oligo(dT)设计引物,但利用全基因中高度分散重复的短序列或回文序列却能有效克服mRNA分子结构的影响,最大限度地扩增全长cDNA;并且这2种引物设计方法还可以提高RNA指纹图谱的重复性,降低反应的假阳性,从而为原核细胞DDRT-PCR引物设计提供新的思路。     

Structural basis for recognition of urokinase-type plasminogen activator by plasminogen activator inhibitor-1

Plasminogen activator inhibitor-1 (PAI-1), together with its physiological target urokinase-type plasminogen activator (uPA), plays a pivotal role in fibrinolysis, cell migration, and tissue remodeling and is currently recognized as being among the most extensively validated biological prognostic factors in several cancer types. PAI-1 specifically and rapidly inhibits uPA and tissue-type PA (tPA). Despite extensive structural/functional studies on these two reactions, the underlying structural mechanism has remained unknown due to the technical difficulties of obtaining the relevant structures. Here, we report a strategy to generate a PAI-1·uPA(S195A) Michaelis complex and present its crystal structure at 2.3-Å resolution. In this structure, the PAI-1 reactive center loop serves as a bait to attract uPA onto the top of the PAI-1 molecule. The P4–P3′ residues of the reactive center loop interact extensively with the uPA catalytic site, accounting for about two-thirds of the total contact area. Besides the active site, almost all uPA exosite loops, including the 37-, 60-, 97-, 147-, and 217-loops, are involved in the interaction with PAI-1. The uPA 37-loop makes an extensive interaction with PAI-1 β-sheet B, and the 147-loop directly contacts PAI-1 β-sheet C. Both loops are important for initial Michaelis complex formation. This study lays down a foundation for understanding the specificity of PAI-1 for uPA and tPA and provides a structural basis for further functional studies.     

Development of a SYBR Green I real-time PCR for quantitative detection of Vibrio alginolyticus in seawater and seafood

AIM: Vibrio alginolyticus is an economically important micro-organism. The main aim of the present study was to develop a real-time polymerase chain reaction (PCR) assay for rapid, sensitive and effective quantification of V. alginolyticus in seawater and seafood. METHODS AND RESULTS: Purified DNA of V. alginolyticus, artificially inoculated seawater and seafood tissue homogenates were subjected to the gyrB-targeted real-time PCR assay. Natural seawater and seafood samples were analysed by this real-time PCR protocol. Specificity tests showed that positive result was obtained only with V. alginolyticus strains. The detection sensitivity was determined to be 0.4 pg of genomic DNA equivalent to 72 cells per PCR in pure culture and 100 cells in 1 ml of seawater or seafood tissue homogenates. Single cell detection is achieved after 3 h of sample enrichment. CONCLUSIONS: A sensitive and specific SYBR Green I-based real-time PCR assay targeting gyrB gene was successfully developed to quantify V. alginolyticus within 6 h in seawater and seafood samples. SIGNIFICANCE AND IMPACT OF THE STUDY: No report on the molecular-based method was available for quantitative detection of V. alginolyticus. This work will provide a novel method for evaluation of the risk of V. alginolyticus to marine environmental health and seafood safety.     

Web-based primer design for single nucleotide polymorphism analysis

The detection of single nucleotide polymorphisms by PCR is necessary for many types of genetic analysis, from mapping genomes to tracking specific mutations. This technique is most commonly used when polymorphisms alter restriction endonuclease recognition sites. Here we describe a web-based program, dCAPS Finder 2.0, that facilitates the design of mismatched PCR primers to create or remove a restriction endonuclease recognition site relative to the polymorphism being analyzed.     

Ligand binding regions in the receptor for urokinase-type plasminogen activator

The interaction between urokinase plasminogen activator (uPA) and its cellular receptor (uPAR) is a key event in cell surface-associated plasminogen activation, relevant for cell migration and invasion. In order to define receptor recognition sites for uPA, we have expressed uPAR fragments as fusion products with the minor coat protein on the surface of M13 bacteriophages. Sequence analysis of cDNA fragments encoding uPA-binding peptides indicated the existence of a composite uPA-binding structure including all three uPAR domains. This finding was confirmed by experiments using an overlapping 15-mer peptide array covering the entire uPAR molecule. Four regions within the uPAR sequence were found to directly bind to uPA: two distinct regions containing amino acids 13--20 and amino acids 74--84 of the uPAR domain I, and regions in the putative loop 3 of the domains II and III. All the uPA-binding fragments from the three domains were shown to have an agonistic effect on uPA binding to immobilized uPAR. Furthermore, uPAR-(154--176) increased uPAR-transfected BAF3-cell adhesion on vitronectin in the presence of uPA, whereas uPAR-(247--276) stimulated the cell adhesion both in the absence or presence of uPA. The latter fragment was also able to augment the binding of vitronectin to uPAR in a purified system, thereby mimicking the effect of uPA on this interaction. These results indicate that uPA binding can take place to particular part(s) on several uPAR molecules and that direct uPAR-uPAR contacts may contribute to receptor activation and ligand binding.     

Distribution of urokinase-type plasminogen activator immunoreactivity in the mouse

Immunocytochemistry, using rabbit antibodies to a urokinase-type 48- Kdalton Mr mouse plasminogen activator, showed that enzyme immunoreactivity is widely distributed in the normal mouse. Strong staining was obtained in widely disseminated connective tissue cells with a fibroblast-like morphology. Such cells occurred in high numbers in the lamina propria mucosae of the gastrointestinal tract, and in moderate numbers in the connective tissue septa of the pancreas. A few such cells were detected around the larynx, trachea, and bronchi. Immunoreactivity also occurred in epithelial cells of the proximal and distal kidney tubules, the ductus deferens, and in pulmonary pneumocytes. In addition, presumably extracellular staining was seen irregularly along the basement membrane and fibrillar structures in the lamina propria of the small and large intestines. Moreover, decidual cells of the mouse placenta stained strongly, and a moderate staining was observed in epithelial cells of involuting mammary glands, but not in those of noninvoluting glands. No immunoreactivity was observed in endothelial cells. Control experiments included absorption of the antibodies against highly-purified mouse plasminogen activator and the corresponding proenzyme, and the finding of a good correspondence between the number of immunoreactive cells and measurable enzymatic activity determined in adjacent tissue sections. Separation by SDS PAGE followed by immunoblotting revealed only one immunochemically stainable protein band with Mr approximately 48 Kdaltons in extracts from tissues showing immunoreactivity.     

A Broadly Reactive One-Step SYBR Green I Real-Time RT-PCR Assay for Rapid Detection of Murine Norovirus

A one-step SYBR Green I real-time RT-PCR assay was developed for the detection and quantification of a broad range of murine noroviruses (MNVs). The primer design was based on the multiple sequence alignments of 101 sequences of the open reading frame (ORF)1−ORF2 junction of MNV. The broad reactivity and quantitative capacity of the assay were validated using 7 MNV plasmids. The assay was completed within 1 h, and the reliable detection limit was 10 copies of MNV plasmid or 0.063 median tissue culture infective doses per milliliter of RAW264 cell culture-propagated viruses. The diagnostic performance of the assay was evaluated using 158 mouse fecal samples, 91 of which were confirmed to be positive. The melting curve analysis demonstrated the diversity of MNV in the samples. This is the first report of a broadly reactive one-step SYBR Green I real-time RT-PCR assay for detecting of MNVs. The rapid and sensitive performance of this assay makes it a powerful tool for diagnostic applications.     

Characterization of the cellular binding site for the urokinase-type plasminogen activator

Human urokinase-type plasminogen activator (uPA) binds rapidly and with high affinity to a number of human cell types; this localizes plasmin generation to the close environment of the cell surface. uPA binding to HeLa and U937 cells is mediated by a single class of sites with an affinity of 3.4 +/- 1.3 x 10(-10) M. Binding is abolished by treatment of the cells with trypsin. Chemical cross-linking of Mr 55,000 125I-uPA to the surface of HeLa and U937 cells with disuccinimidyl suberate or with formaldehyde results in the formation of a labeled complex of Mr 100,000, suggesting a Mr of 45,000 +/- 5,000 for the receptor or a subunit thereof. When cells solubilized in Triton X-114 are subjected to heat-induced phase separation, unoccupied receptor, receptor-bound 125I-uPA, and cross-linked 125I-uPA-receptor complex all partition in the detergent phase, whereas the unbound ligand remains in the aqueous phase; similar phase partitioning is observed with endogenous uPA-receptor complexes from cultured human and murine cells. Thus, uPA bound at the cell surface is tightly associated with an amphiphilic membrane protein. Interaction of uPA with this plasma membrane receptor is species-specific, since human uPA fails to bind to murine cells, and murine uPA does not bind to human cells. Finally, incubation of HeLa cells in the presence of epidermal growth factor or phorbol 12-myristate 13-acetate results, over a period of 24 h, in a progressive change in uPA binding: an approximately 10-fold increase in the number of sites is accompanied by a 10-fold decrease in their affinity. Cross-linking and phase partitioning of 125I-uPA bound to epidermal growth factor- or phorbol 12-myristate 13-acetate-treated cells indicate that, as in control conditions, it is associated with a Mr 45,000 cell surface amphiphilic polypeptide.