甲肝病毒减毒株(H2)RNA的全长RT-PCR扩增

通过RT-PCR技术扩增了甲肝病毒减毒株(H₂)全长RNA,并对长片段RT-PCR扩增进行了方法学上的探讨.采用抗血清特异沉淀病毒;盐酸胍-酸性酚、氯仿一步法分离纯化病毒RNA,可得到高质量的RNA样品;以此RNA为模板,在无RNA酶的逆转录酶作用下,合成单链cDNA;继续以此cDNA为模板,利用32 mer寡核苷酸引物, 在Taq和Deep Vent DNA多聚酶的作用下进行PCR扩增,得到7.4 kb的扩增产物.     

两种微量RNA扩增方法的比较研究

本研究通过比较体外转录和单引物扩增这两种扩增微量RNA的不同方法,以寻找一种高效的扩增方法。我们用两种不同方法分别扩增小鼠大脑全皮层及第五皮层细胞的RNA,扩增的RNA合成cDNA后进行荧光定量PCR实验,根据PCR结果比较两种不同扩增方法的效率。WT-ovation扩增RNA的效率约为IVT效率的2.8倍;IVT方法扩增后,基因D-C值与引物距离mRNA 3'端的长度及mRNA的长度均存在正线性相关(P<0.05),即引物距离mRNA的3'端越近、mRNA越短,基因D-Ct值越低。而WT-ovation方法扩增后,基因D-Ct值与引物距离mRNA 3'端的长度及mRNA的长度均不存在统计学相关性。与IVT方法相比,WT-ovation方法效率更高,扩增时受影响因素较少、更稳定。     

NASBA(依赖核酸序列的扩增)及其在病毒检测中的应用

NASBA(nucleic acid sequence based amplification)即依赖核酸序列的扩增技术,是一种扩增RNA的新技术,是由一对引物介导的、连续均一的、体外特异核苷酸序列等温扩增的酶促反应过程。反应在42℃进行,可以在2h左右将模板RNA扩增约109~12倍,不需特殊的仪器。NASBA已经广泛应用于细菌、病毒等多种病原微生物的检测,就NASBA的技术原理及其在病毒检测中的应用作一综述。     

一种用于基因芯片可靠的RNA线性扩增技术

基因芯片是大规模表达谱分析的有力工具 ,有助于阐明疾病发生的分子机制及发现新的诊治靶标。但常规方法需要大量RNA ,每张芯片需要 5 0～ 2 0 0 μg总RNA ,2～ 5 μgmRNA。许多珍贵难得样本都不能满足这一要求 ,成为限制芯片广泛应用的瓶颈。结合模板转移效应 ,优化了基于T7的RNA线性扩增技术 ,可从 3μg以下总RNA得到足量的反义RNA ,克服了这一难题。同一RNA样本的自身比较试验结果显示反义RNA标记的芯片与总RNA、mRNA标记的芯片假阳性率相似。同一对RNA样本的表达谱分析也显示反义RNA标记的芯片与总RNA、mRNA标记的芯片无明显差异。     

利用优化的5′-RACE实验定位副溶血弧菌基因的转录起始位点

目的:优化5′-cDNA末端快速扩增(5′-RACE)实验平台,用于定位副溶血弧菌(VP)基因的转录起始位点。方法:提取VP的总RNA,用rDNaseⅠ消化去除可能污染的基因组DNA;利用T4 RNA连接酶将已知序列的寡核苷酸片段连接至RNA的5′端,进而将其逆转录成cDNA;以cDNA为模板,采用巢式PCR技术扩增目的基因DNA片段,并将其直接克隆入T载体;最后通过测序比对的方法确定靶基因的转录起始位点。利用引物延伸实验进一步研究VPA1027的转录起始位点,以检验5′-RACE实验结果的可靠性。结果:5′-RACE实验结果表明,VPA1027、scrG、scrA、cpsA及VPA0198的转录起始位点分别为G(-103)、G(-70)、T(-205)、C(-129)和G(-238)(翻译起始位点为+1);引物延伸结果显示,VPA1027的转录起始位点也为G(-103)。结论:优化后的5′-RACE实验可以精确定位VP基因的转录起始位点。     

一种用于基因芯片可靠的双轮RNA线性扩增技术

DNA微阵列能在一次实验中检测成千上万个基因的表达情况, 有助于阐明疾病发生的分子机制及发现新的诊治靶标.但常规方法需要大量RNA, 因而基于T7 RNA线性扩增技术逐渐成为微阵列表达谱实验中最常用的探针制备方法.本方法将实验步骤进一步改进,增加额外的一轮体外转录,并结合Klenow酶标记技术来制备cDNA靶标和寡核苷酸芯片杂交.从纳克量级的总RNA起始,本方法和常规的RNA单轮线性扩增法相比,仍然准确地保留了约70%的基因表达信息.同一RNA样本的自身比较实验及重复实验结果也显示,该方法具有较高的可靠性和重复性.RNA双轮体外扩增法需要的起始RNA相对于常规的单轮扩增法减少了很多（10 ng甚至更少）,因而非常适合分析那些只能提供微量RNA的样本.     

核酸恒温扩增技术研究进展

核酸恒温扩增技术在生命科学研究及相关诸多领域已经得到了广泛应用。我们对核酸恒温扩增技术的最新进展作一简要综述,包括环介导恒温扩增、链替代扩增、依赖核酸序列的扩增、滚环扩增、切口酶核酸恒温扩增、依赖解旋酶的恒温扩增、转录依赖的扩增、杂交捕获法、转录介导的扩增等的原理、优缺点及应用。     

乙脑病毒全长cDNA的扩增克隆及体外转录制备感染性RNA的研究

本研究根据已知的乙脑病毒(JEV)SA14株基因序列设计一套引物 ,利用长模板RT-PCR 技术,一次扩增出了JEV的全长cDNA,并采用大片段克隆技术将其克隆于载体的RNA聚合酶启动子下游.阳性克隆转录的RNA转染HBK细胞后细胞产生病变,经乳鼠脑内接种及特异性免疫荧光染色证明为JEV,这一结果表明JEV感染性克隆的构建获得了成功.其次,合成一条含有 RNA聚合酶启动子序列的5′引物,利用长模板RT-PCR方法扩增出带有启动子的JEV全长cDNA ,以此cDNA为模板作体外转录.转录产物转染BHK细胞后观察到了典型的JEV病变.收获的病毒经乳鼠脑内接种及免疫荧光染色证明为JEV,从而建立了制备JEV感染性RNA的快捷方法.本研究构建的JEV感染性克隆与建立的长模板RT-PCR快速制备JEV感染性RNA的方法,将为JEV 分子生物学研究的后续工作提供有力的工具和奠定坚实的基础.     

RT-PCR克隆人纤溶酶cDNA大片段

目的:以人胎儿肝脏总RNA为模板,克隆人纤溶酶(plasmin)cDNA大片段。方法:采用异硫氰酸胍一步法提取总RNA,RT-PCR技术获取目的基因。结果:成功地扩增出1.74kb的人纤溶酶基因,并研究了扩增人纤溶酶cDNA大片段的特定实验条件。结论:为克隆cDNA大片段研究提供了简便、快速的方法。     

利用PCR技术构建体外高效转录系统

设计并合成了一对 PCR 反应引物,其5′端引物除含有目的基因5′端序列外,还外加 T7 RNA 聚合酶启动子的17个核苷酸.3′端引物则按常规设计.以染色体 DNA为模板,通过 PCR,可扩增出带有 T7 RNA 聚合酶启动子的目的基因 DNA 片段.以此 PCR 产物为模板,在体外成功实现了高效转录.这是一种快速、简便构建体外高效转录系统的好方法.     

Intercalation activating fluorescence DNA probe and its application to homogeneous quantification of a target sequence by isothermal sequence amplification in a closed vessel

We developed a completely homogeneous and isothermal method of detecting RNA sequences and demonstrated ultrarapid and direct quantification of pathogenic gene expression with high sensitivity. The assay is based on performing isothermal RNA sequence amplification in the presence of our novel DNA probe, an intercalation activating fluorescence DNA probe, and measuring the fluorescence intensity of the reaction mixture. When detecting mecA gene expression of methicillin-resistant Staphylococcus aureus, we quantified starting copies ranging from 10 to 10(7) copies within 10min. The primer sequences were designed to bind to secondary structure-free sites of the target RNA, which enabled a totally isothermal protocol to quantify mRNA specifically in a sample of existing genomic DNA. When we applied this to quantifying the expression of marker genes of Vibrio parahaemolyticus and Mycobacterium bovis BCG strain, the results correlated well with the viability of each bacterium. We also demonstrated monitoring Pab gene expression of M. bovis BCG during cultivation with antibiotics. The present method can potentially realize rapid antimicrobial susceptibility testing of slowly growing organisms, such as tuberculosis.     

土壤微生物总活性研究方法进展

微生物总活性是指在某一时段内微生物所有生命活动的总和,它直接决定着微生物行使生理、生态功能的能力,是微生物学研究的热点,也是难点。迄今为止,还没有建立直接测定微生物总活性的方法,只能用一些相关指标来间接反映它。目前常用的指标主要包括微生物的呼吸速率、生长速率以及胞内RNA含量等。与其它一些基质和环境相比,测定土壤中的微生物总活性更为困难。通过总结研究土壤微生物总活性常用的3种方法,在简略概括传统的土壤微生物呼吸测定法的基础上,详细介绍了放射性同位素标记法和RNA直接表征法的原理和操作流程,整理归纳了一些重要应用案例,比较分析了不同方法的优缺点,以期为选择研究土壤微生物总活性的适宜方法提供依据。     

Genotyping of phenotypically defined cells in neoplasia: enhanced immunoFISH via tyramide signal amplification (TSA) segregates immunophenotypically—defined cell populations for gated genotyping

Molecular morphologic tools exist for simultaneously visualizing immunophenotype and genotype of tumors, but are frequently hampered by a delicate balance between removing sufficient amount of the protein blocking full access of the probe to hybridize to target nucleic acids while still preserving sufficient target antigen for immunophenotyping. The result is often suboptimal, with either insufficiently visualized gene deletions and amplifications due to masking protein, or overdigestion of the protein target. Our purpose was to design and validate a gated genotyping assay that enables optimal and concomitant detection of both gene and protein. Using the proliferating endothelial cell compartment within gliomas organized in a tissue microarray (TMA), we tested the hypothesis that tyramide signal amplification (TSA) with deposition of a fluorochrome could be used during immunophenotyping, permitting sufficient protein digestion while insuring probe accessibility to nucleic acid target. The method was successfully validated using a TMA containing 38 glioma cases previously genotyped for EGFR amplification. CD31 positive endothelial cells were segregated via TSA-based Alexa-Fluor 647 immunofluorescence for analysis of EGFR amplification of the gliomas organized in the TMA. Enhanced immunoFISH (TSA) successfully segregates immunophenotypically—defined cell populations for gated genotyping.     

滚环扩增技术的原理及其应用的研究

滚环扩增是近年来发展起来的一种恒温核酸扩增方法。这种方法不仅可以直接扩增DNA和RNA,还可以实现对靶核酸的信号放大,灵敏度达到一个拷贝的核酸分子,因此,RCA技术在全基因组扩增、单核苷酸多态性、DNA芯片、蛋白质芯片等方面检测中具有很大的应用价值和潜力。     

Expanding the utility of heptamer-type sgRNA for TRUE gene silencing

tRNase Z(L)-utilizing efficacious gene silencing (TRUE gene silencing) is a novel technology for suppressing gene expression. TRUE gene silencing is based on a unique enzymatic property of mammalian tRNase Z(L), which is that it can cleave any target RNA at any desired site by recognizing a pre-tRNA-like or micro-pre-tRNA-like complex formed between the target RNA and artificial small guide RNA (sgRNA). sgRNA is divided into four groups, 5'-half-tRNA, RNA heptamer, hook RNA, and ～14-nt linear RNA. One of the final destinations of TRUE gene silencing is to generate cancer therapeutic sgRNAs, and from a pharmacological point of view, heptamer-type sgRNA appears to be the most appropriate for this purpose. In this paper, we present two strategies to expand the utility of heptamer-type sgRNA: one is about locked nucleic acid (LNA) modifications of heptamers and the other is about usage of double heptamers. We showed that RNA heptamers with LNA modifications can work as sgRNA in vitro and in vivo. We also demonstrated that two consecutively aligned heptamers can guide target RNA cleavage by human tRNase Z(L) as efficiently as a corresponding 14-nt sgRNA in vitro and that a double heptamer can work much better than a 14-nt sgRNA in vivo.     

A cloned unique gene of drosophila melanogaster contains a repetitive 3′ exon whose sequence is present at the 3′ ends of many different mRNAs

We have started to study a cloned genomic DNA fragment ～7 kb long (denoted as H55) from the 7B3-4 region in the X chromosome of Drosophila melanogaster. The major part of the fragment is a single-copy sequence. It directs the synthesis of mRNA that makes up ～0.1% of the cytoplasmic poly(A)⁺ RNA from Drosophila embryos. The H55 gene is split by an intervening sequence, yielding a large single-copy exon and a small repetitive 3′ exon represented by hundreds of copies in the genome. This repetitive sequence (“suffix”) is also present at the 3′ ends of ～2% of all cytoplasmic poly(A)⁺ RNA chains.     

Expression of endogenous avian myeloblastosis virus information in different chicken cells.

Uninfected chicken cells were found to contain endogenous avian myeloblastosis virus (AMV)-specific information. Different tissues from chicken embryos and chickens expressed different amounts of the AMV-specific information. The endogenous AMV-related RNA was most abundant in bone marrow cells, which contained about 20 copies per cell. About 5 to 10 copies of AMV endogenous RNA per cell were found in embryonic yolk sac cells and bursa cells. The spleen, muscle, liver, and kidney cells of chickens and the fibroblasts of chicken embryos contained about two copies per cell. The amounts of AMV endogenous RNA in bone marrow, yolk sac, and bursa varied with age. From 19-day-old embryos to 2-week-old chickens, the bone marrow contained 20 copies of AMV RNA per cell. Bone marrow cells from 2-year-old chickens contained five copies per cell. Yolk sac cells of 10-day-old embryos and 1-day-old chickens were found to contain two copies per cell, whereas in 15- to 17-day-old embryos, these cells contained 5 to 10 copies. These results indicate that the level of endogenous AMV expression correlates with the development of granulopoiesis of the chicken hemopoietic system. The results of experiments on the thermostability of RNA-DNA hybrids indicated that the endogenous AMV RNA is closely related to viral AMV RNA. The expression of endogenous AMV information is independent of the activity of the chick helper factor. This endogenous AMV information is expressed as 20 to 21S RNA in both bone marrow and yolk sac cells.