PCR扩增试验的动力学数学模型

PCR技术已日趋成熟,但因为影响因素较多、反应过程比较复杂,直到目前PCR技术已创立近二十年,尚未能给出较好的描述PCR 反应的数学方法。我们根据它的基本原理提出了能够描述其反应过程的动力学方程：Wamp=［Ntarg×(1+P)n1+0.5×Cenz×U×P×Ceactiv×(n-n1)-Ntarg× (1+n×P)］×Cu×M,准确地描述了PCR反应的产物积累规律,建立了PCR反应的动力学数学模型。用动力学数学模型预测的PE 7700仪器的CT值与仪器的实际数值一致。动力学数学模型配合适当的监测设备可以构成自动化的PCR 定量仪器。PE 7700 仪器使用本动力学模型处理、分析数据,定量结果的准确性会更好。各实验室可根据各自的实验条件,由模型估算PCR产物数量,为PCR后产物继续处理提供较准确的数量信息。本模型阐明了PCR反应在多次循环后必然由指数扩增转变为线性扩增的分子基础,为定量PCR 提供了准确的计算方法。 Abstract:The PCR technique has been set up for nearly twenty years and is becoming more and more ripe.But because of the multiple influencing factors and complicated reaction procedures,no mathematical method that can describe the PCR reaction has been given.On the basis of its elementary principle,we suggested a kinetic equation to describe the reaction procedure,Wamp=［Ntarg×(1+P)n1+0.5×Cenz×U×P×Ceactive×(n-nl)-Ntarg×(1+n×P)］×Cu×M.This equation can describe correctly the accumulation rule of PCR product and thus build up the kinetic-mathematical model of PCR reaction.The predicted CT value of PE 7700 by the kinetic-mathematical model was in accordance with the real value detected by the machine.This kinetic-mathematical model accompanied by proper detecting equipment and computer could make an automatic PCR instrument,which would produce much better result.A laboratory can predict the amount of PCR product by this model and provide accurate information for further handling of PCR product according to its own condition.In this model,the molecular basis that PCR reaction is doomed to change from exponential amplification to linear amplification had been clarified.     

PCR一步法构建融合蛋白基因fpg

采用一种不需要限制核酸酶和连接酶的新方法——“PCR一步法”将芳香烃化合物降解的关键基因pheB和绿色荧光蛋白编码基因gfp融合,构建得到融合蛋白基因fpg。该方法在一个PCR反应体系中通过三个引物、两个模板扩增得到一个含有中间柔性肽段-Gly4Ser-的融合基因fpg。本文研究结果表明,PCR一步法是一种快速方便的构建融合基因的方法。Abstract: TP-PCR,a method developed for fusion gene construction without the use of endonuclease and ligase, was performed to construct a fused fpg gene. The TP-PCR reaction system contained three primers and two templates and resulting PCR product, fused fpg gene, consisted of three sections: pheB gene, which was responsible for catechol 2,3-dioxygenase, gfp gene for GFP protein and the intermediate ligation segment which was designed for the correct expression of the fusion gene. The result in this paper showed that the TP-PCR method is one of rapid and convenient methods for fused gene construction.     

Quantitative genetic analysis of chlorophyll a fluorescence parameters in maize in the field environments

Chlorophyll fluorescence transient from initial to maximum fluorescence("P" step) throughout two intermediate steps("J" and "I")(JIP‐test) is considered a reliable early quantitative indicator of stress in plants. The JIP‐test is particularly useful for crop plants when applied in variable field environments. The aim of the present study was to conduct a quantitative trait loci(QTL) analysis for nine JIP‐test parameters in maize during flowering in four field environments differing in weather conditions. QTL analysis and identification of putative candidate genes might help to explain the genetic relationship between photosynthesis and different field scenarios in maize plants. The JIP‐test parameters were analyzed in the intermated B73 Mo17(IBM) maize population of 205 recombinant inbred lines. A set of 2,178 molecular markers across the whole maize genome was used for QTL analysis revealing 10 significant QTLs for seven JIP‐test parameters, of which five were co‐localized when combinedover the four environments indicating polygenic inheritance and pleiotropy. Our results demonstrate that QTL analysis of chlorophyll fluorescence parameters was capable of detecting one pleiotropic locus on chromosome 7, coinciding with the gene gst23 that may be associated with efficient photosynthesis under different field scenarios.     

Analyzing the biology on the system level

Although various genome projects have provided us enormous static sequence information, understanding of the sophisticated biology continues to require integrating the computational modeling, system analysis, technology development for experiments, and quantitative experiments all together to analyze the biology architecture on various levels, which is just the origin of systems biology subject. This review discusses the object, its characteristics, and research attentions in systems biology, and summarizes the analysis methods, experimental technologies, research developments, and so on in the four key fields of systems biology--systemic structures, dynamics, control methods, and design principles.     

实时定量PCR技术及应用

实时定量PCR(Real-tim e Quantitative Polym erase Chain Reaction,RQ-PCR),是20世纪90年代中期发展起来的基于PCR技术的利用不同的荧光检测来给核酸定量的技术。克服了传统PCR的许多不足,能准确敏感地检测模板浓度,DNA拷贝数和检测基因变异。综述了RQ-PCR技术的原理,RQ-PCR实时定量检测系统及应用。     

番茄叶片基因组DNA快速制备技术及其在基于实时荧光定量PCR的转基因检测中的应用

以番茄(Solanum lycopersicum L.cv.Micro-Tom)叶片为试材,建立了一种简便快速制备叶片基因组DNA的方法。2~20 mm2的叶片即可满足制备要求,制备过程只需一种提取试剂、只涉及1次移液和1次离心操作,不涉及沉淀。确定了所制备的DNA用于实时荧光定量PCR的合适用量为0.1~0.2μL(反应总体积为12.5μL),发现过量模板的使用可降低PCR效率且可导致扩增失败。该项DNA快速制备及相适应的实时荧光定量PCR技术已成功应用于番茄转基因植株检测。     

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。     

实时荧光定量PCR在固氮酶基因检测中的应用

实时荧光定量PCR是近年发展起来的一种新的实时定量检测特定核酸技术,它是核酸探针技术、荧光共振能量传递技术和PCR技术的有机结合。与常规PCR相比,它具有特异性更强、能有效解决PCR污染问题、自动化程度高等特点,扩大了PCR的应用范围。概述实时荧光定量PCR技术在固氮酶(nifH)基因检测中的应用与研究进展,并探讨该技术的发展和应用前景。     

实时定量PCR技术及其应用

实时定量PCR(Real—time Quantitative Polymerase Chain Reaction,RQ—PCR)技术是20世纪90年代中期发展起来的一种新型核酸定量技术。该技术具有实时监测、快速、灵敏、精确等特点,是对原有PCR技术的革新,扩大了PCR的应用范围。本文综述了RQ—PCR技术的原理、RQ—PCR仪、RQ—PCR实时定量检测系统及其应用。     

Event-specific qualitative and quantitative PCR methods for the detection of genetically modified rapeseed Oxy-235

Oxy-235 is an oxynil-tolerant genetically modified rapeseed approved for commercialized planting in Canada. The aim of this study was to establish event-specific qualitative and quantitative detection methods for Oxy-235. Both the 5'- and 3'-junction sequences spanning the plant DNA and the integrated gene construct of the Oxy-235 event were isolated, sequenced and analyzed. A 1298-bp deletion of the rapeseed genomic DNA that showed a high similarity to the mRNA sequence of Arabidopsis thaliana was found in the integration site of the insert DNA. Event-specific qualitative PCR methods were established, with one method producing a 105-bp product specific for the 5'-integration junction and the other method producing a 124-bp product specific for the 3'-junction. The absolute detection limits for the qualitative PCR were determined to be 100 initial template copies for the 5'-junction and ten for the 3'-junction. Quantitative methods were also developed that targeted both of the junction fragments. The limit of detection of the quantitative PCR analysis was ten initial template copies for either the 5'- or 3'-junction, while the limit of quantification was determined to be approximately 50 initial template copies. The real-time PCR systems so established were examined with two mixed rapeseed samples with known Oxy-235 contents and found to obtain the expected results.     

数字PCR仪校准方法研究

数字PCR仪是核酸绝对定量的重要仪器,因此确保数字PCR仪检测结果的准确性十分重要。通过对国内市场上数字PCR仪的比较分析,剖析了数字PCR仪的性能指标,对数字PCR仪的校准方法进行了探讨,设定了拷贝数浓度相对示值误差、拷贝数浓度重复性、荧光通道一致性和反应单元个数重复性作为数字PCR仪整机校准的计量技术指标,采用具有溯源性的国家有证标准物质,对方法进行了试验验证。验证结果表明了校准思路和方法的可行性,该方法操作性强,能够满足仪器技术要求以及用户需求, 提高了数字PCR仪检测结果的准确性和可靠性,对进一步拓展和深化数字PCR 技术的应用具有积极的促进作用。     

Calibration-curve-free quantitative PCR: a quantitative method for specific nucleic acid sequences without using calibration curves

We have developed a simple quantitative method for specific nucleic acid sequences without using calibration curves. This method is based on the combined use of competitive polymerase chain reaction (PCR) and fluorescence quenching. We amplified a gene of interest (target) from DNA samples and an internal standard (competitor) with a sequence-specific fluorescent probe using PCR and measured the fluorescence intensities before and after PCR. The fluorescence of the probe is quenched on hybridization with the target by guanine bases, whereas the fluorescence is not quenched on hybridization with the competitor. Therefore, quench rate (i.e., fluorescence intensity after PCR divided by fluorescence intensity before PCR) is always proportional to the ratio of the target to the competitor. Consequently, we can calculate the ratio from quench rate without using a calibration curve and then calculate the initial copy number of the target from the ratio and the initial copy number of the competitor. We successfully quantified the copy number of a recombinant DNA of genetically modified (GM) soybean and estimated the GM soybean contents. This method will be particularly useful for rapid field tests of the specific gene contamination in samples.     

Basic principles of quantitative PCR

The polymerase chain reaction (PCR) is an extremely sensitive method owing to the repetitive multiplication of template molecules. This property is a drawback for quantitative measurements because small differences in the multiplication factor lead to large differences in the amount of product. Two methods can be used to solve the problem of quantification: kinetic methods based on the determination or comparison of the amplification factor; and coamplification methods, which compare the amount of product to that of a simultaneously amplified standard template. An overview of the theoretical background of both methods is presented. For selection of a suitable method, both theoretical and practical considerations are important. Kinetic methods are the most convenient if PCR can be performed without opening the tubes, as in some apparatus using fluorescence detection. Coamplification methods can be done without expensive equipment but requires the parallel running of several PCR tubes. When the number of initial template molecules is close to one, as in the limiting dilution technique, statistical considerations become important.