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技术在鱼类病害研究中的应用

实时荧光定量PCR技术是一种新的核酸定量技术,通过检测PCR产物中荧光信号强度达到定量的目的,与常规PCR相比,具有无污染、特异性强、检测灵敏、定量准确等特点,该技术在分子诊断、动植物检疫等方面得到了广泛的应用.目前水产养殖业处于飞速发展时期,其中鱼类的病害问题也日益突出,为了预防和控制鱼类病害,实时荧光定量PCR技术已逐渐应用于鱼类病害的研究中.该文将从实时荧光定量PCR的技术原理、主要类型以及实时荧光定量PCR技术在鱼类病害研究的应用研究作一综述.     

实时荧光定量PCR及其在传染性疾病检测中的应用

实时荧光定量PCR技术被广泛应用于实验研究、临床检测中。与普通的PCR相比,实时荧光定量PCR技术具有特异性强、灵敏度高、重复性好、定量准确、速度快、全封闭反应等优点。我们综述了实时荧光定量PCR技术的原理、定量方法,及其在传染性疾病检测研究中的应用。     

荧光定量PCR 方法及分子标志物在海洋污染监测中的应用进展

荧光定量PCR 作为一种核酸定量技术, 可在PCR 扩增时在体系中加入荧光染料或荧光基团, 实时监测荧光信号从而对PCR 扩增产物进行实时准确定量, 技术灵敏度高, 特异性强。通过对荧光定量PCR 的原理、分类、优缺点及几种定量分析方法对比进行简述, 并对其在国内外海洋环境污染监测中的广泛应用和研究进行了全面综述, 从而对荧光定量PCR 和分子标志物在海洋监测中的应用前景做进一步的展望。     

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。     

实时定量PCR技术的介绍

实时定量PCR(real-timePCR)技术是近几年发展起来的新技术 ,既保持了PCR技术灵敏、快速的特点 ,又克服了以往PCR技术中存在的假阳性污染和不能进行准确定量的缺点。另外 ,还有重复性好、省力、低费用等优点。实时定量PCR技术是从传统PCR技术发展而来 ,其基本原理是相同的 ,主要不同之处是其定量的体系。下面简单介绍一下该技术定量的原理。1　荧光染料的应用荧光染料的应用是实时PCR技术能够进行定量检测的一个重要部分 ,在PCR反应体系中应用荧光标记物 ,通过监测荧光信号的累积实现对整个PCR循环进程的观察。目前主要有四种方法…     

实时荧光定量PCR及其在微生物生态学中的应用

定量描述微生物群落的组成,在微生物生态学的许多研究领域都是非常重要的。然而由于可培养技术的局限性,定量描述微生物群落成为比较困难的事情。最近包括PCR技术在内的分子生物学技术为人们提供了有力的工具,使对微生物群落的分布、丰度等有了进一步的了解。实时荧光定量PCR技术作为核酸定量检测技术,自从发明以来在微生物生态学研究中逐渐得到了广泛的应用。从微生物生态学角度,综述了实时荧光定量PCR技术的原理、发展、优缺点及其在微生物生态学研究中的应用与研究进展,并探讨了实时荧光定量PCR技术的发展和应用前景。     

实时荧光定量PCR(TaqMan)法测定外源基因的拷贝数

实时荧光定量PCR是近年新兴的一项技术,因其快速、方便、便宜,需要DNA样品量少,无需放射性检测等优点被广泛应用于基因的定量分析。该文就实时荧光定量PCR(TaqMan)技术的发展、基本原理及测定外源基因拷贝数的技术流程做一介绍。     

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.     

Quantitative precision of an automated, fluorescence-based image cytometer.

Digital image-based cytometry of clinical specimens labeled with fluorescent, disease-specific markers holds promise for becoming an important diagnostic and prognostic technique because the technique can make a diverse range of quantitative biochemical, morphologic, densitometric and contextual measurements on intact specimens. It has been previously shown by us, using an image cytometer (IC) consisting entirely of commercially available components, that the nuclei of individual cells in slide-supported specimens can be detected automatically using a fluorescent DNA stain and image analysis software. The purpose of this study was to determine the precision of the IC for quantifying the integrated fluorescence intensity and area of fluorescent standard beads and nuclei. Integrated intensities could be quantified to between 2.3% and 3.5% precision using a 40x objective lens and between 1.6% and 2.3% using a 20x objective. The main contribution to this uncertainty was 2% inaccuracy in determining the variations in sensitivity over the imaging area. Areas could be quantified to between 0.91% and 2.1% using a 40x objective and between 2.8% and 3.2% using a 20x objective. Significant quantification errors were introduced if the objects were not in focus or were touching each other. Overall, however, these results demonstrated that image cytometry of fluorescence-stained specimens can yield quantitative results with sufficient precision for determining DNA ploidy distributions and for making other measurements on clinical specimens.     

Limitation of usage of PicoGreen dye in quantitative assays of double-stranded DNA in the presence of intercalating compounds

PicoGreen is a very sensitive fluorescent dye for quantitative assays of double-stranded DNA (dsDNA) in solution and is used in several analytical protocols in which sensitive and precise DNA detection is needed, also for examination of drug-DNA interactions. The data shown in this paper indicate that compounds intercalating to DNA influence the applicability of PicoGreen dye for quantitative measurements of dsDNA, and for this reason PicoGreen dye is not suitable for examination of drug-DNA interactions, especially interstrand DNA crosslinks.     

Refined quantitative fluorescent PCR of Y-chromosome DNA sequences mosaics in Turner's syndrome patients--alternative to real-time PCR

BACKGROUND: Real-time polymerase chain reactions (PCRs) are the most frequently used techniques for gonosomal mosaics quantification. The primary aim of this work is to assess and optimize the refined technique of quantitative fluorescent polymerase chain reaction (RQF PCR) in the quantification of Y-chromosome sequences in gonosomal mosaics. The method was applied to the analysis of Y-chromosome sequences (amelogenin gene, AMELX/Y-loci) in peripheral lymphocytes and gonadal tissues in Y-positive Turner's syndrome (TS) patients. METHODS: RQF PCR was used for molecular quantification, and fluorescent in situ hybridization (FISH) technique was used for comparison. RESULTS: Based on a formulated calibration curve, DNA mosaics from six Y-positive patients and gonads from one patient were deducted. For calculation of rare mosaics, it is possible to take advantage of a new empirical formula. FISH results were comparable to RQF PCR. CONCLUSION: The sensitivity of RQF PCR brings significant progress in the analysis of gonosomal aberrations. RQF PCR also finds applications in prenatal diagnostics of maternal contaminations of amniotic fluid and foetal DNA in maternal blood and analysis of chimerism in patients after bone marrow transplantation. The method is very convenient for determining the number of testis-specific protein, Y-linked (TSPY) gene repetitions.     

Quantitative fluorescenct analysis of different conformational forms of DNA bound to the dye, 4′,6-diamidine-2-phenylindole,and sepasated by gel electrophoresis

A quantitative fluorescent method for estimating the amounts of different conformational forms of the same DNA on agarose gels is described. Supercoiled, open circular, and linear forms of PM2 DNA and fluorescent dye (4′,6-diamidine-2-phenylindole) were used. The results are compared with respective radiometric estimations and are shown to be highly reproducible.     

对果蝇S期细胞内组蛋白基因的原位定量分析

利用微型计算机控制的荧光显微镜、荧光强度检测仪和图像记录装置并结合荧光原位杂交法对果蝇细胞核内组蛋白基因的复制时期进行了研究,从而建立了一套细胞内直接定量分析的方法。根据果蝇胚胎原代培养细胞核的DAPI染色强度确定处于S期的细胞。用杂交信号的荧光强度与细胞核荧光强度的相关关系来反映组蛋白基因的复制时期。结果表明果蝇组蛋白基因的复制是在DNA合成早期进行的。这套方法至少可直接在细胞上对每套基因组100以上拷贝数的熏复DNA序列进行有效的定量分析。     

Application of fetal DNA detection in maternal plasma: a prenatal diagnosis unit experience.

Non-invasive prenatal diagnosis tests based on the analysis of fetal DNA in maternal plasma have potential to be a safer alternative to invasive methods. So far, different studies have shown mainly fetal sex, fetal RhD, and quantitative variations of fetal DNA during gestation with fetal chromosomal anomalies or gestations at risk for preeclampsia. The objective of our research was to evaluate the use of fetal DNA in maternal plasma for clinical application. In our study, we have established the methodology needed for the analysis of fetal DNA. Different methods were used, according to the requirements of the assay. We have used quantitative fluorescent polymerase chain reaction (QF-PCR) to perform fetal sex detection with 90% sensitivity. The same technique permitted the detection of fetal DNA from the 10th week of gestation to hours after delivery. We have successfully carried out the diagnosis of two inherited disorders, cystic fibrosis (conventional PCR and restriction analysis) and Huntington disease (QF-PCR). Ninety percent of the cases studied for fetal RhD by real-time PCR were correctly diagnosed. The detection of fetal DNA sequences is a reality and could reduce the risk of invasive techniques for certain fetal disorders in the near future.     

Fate of plasmids containing Mu DNA: chromosome association and mobilization

Summary The fluorescent dye, diamidinophenylindole-dihydrochloride (DAPI) can be added to CsCl gradients to enhance the density resolution of DNA species, independent of their topological configurations. When Proteus mirabilis and Escherichia coli strains carrying an RP4::Mucts plasmid were examined with the use of such a technique, it was found that after thermal induction of the prophage essentially all of the plasmid DNA became associated with the chromosome. This quantitative association is detergent-RNase-and pronase-resistant and dependent on the expression of Mu genes. The association is temporally, and probably functionally, correlated with the onset of Mu DNA replication. Genetic studies with F'::mini Mu plasmids indicate that some of the association results in stable Hfr formation, and does not require the product of Mu gene B.     

Rapid detection of trisomies 21 and 18 and sexing by quantitative fluorescent multiplex PCR

Aneuploidies involving chromosomes 21, 18, 13, X and Y account for over 95% of all chromosomal abnormalities in live-born infants. Prenatal diagnosis of these disorders is usually accomplished by cytogenetic analysis of amniotic or chorionic cells but this is a lengthy procedure requiring great technical expertise.In this paper, we assess the diagnostic value of using a quantitative fluorescent polymerase chain reaction (PCR) suitable for the simultaneous and rapid diagnosis of trisomies 21 and 18 together with the detection of DNA sequences derived from the X and Y chromosomes. Samples of DNA, extracted from amniotic fluid, fetal blood or tissues, and peripheral blood from normal adults were investigated by quantitative fluorescent PCR amplification of polymorphic small tandem repeats (STRs) specific for two loci on each of chromosomes 21 and 18. Quantitative analysis of the amplification products allowed the diagnosis of trisomies 21 and 18, while sexing was performed simultaneously using PCR amplification of DNA sequences derived from the chromosomes X and Y. These results indicate the advantages of using two sets of STR markers for the detection of chromosome 21 trisomies and confirmed the usefulness of quantitative fluorescent multiplex PCR for the rapid prenatal diagnosis of selected chromosomal abnormalities. Received: 23 January 1996 / Revised: 21 February 1996