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。     

实时定量PCR检测新生儿全血中肺炎克雷伯菌方法的建立和应用

目的:建立实时定量PCR(RQ-PCR)快速检测新生儿血液标本中肺炎克雷伯菌基因组DNA的方法,并进行初步临床应用。方法:选择肺炎克雷伯菌高度保守的二鸟苷酸环化酶基因作为靶基因,设计特异性引物和TaqMan探针,建立RQ-PCR反应体系;采用含靶基因扩增片段的重组质粒建立标准曲线,提取血液中的基因组DNA,对500份新生儿血液标本进行RQ-PCR检测。结果:设计的引物和探针特异性高,检测限为1个拷贝数;500份新生儿血液标本中,RQ-PCR检测为阳性的有18个病例,阳性率为3.6%,明显高于血培养的阳性率2.4%(12个病例),差异具有统计学意义(P0.01)。结论:RQ-PCR可用于检测新生儿血液标本中的肺炎克雷伯菌,此方法快速、灵敏、特异性强。     

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。     

实时荧光定量PCR的发展和数据分析

实时荧光定量PCR技术是基因时代一项用于检测mRNA的常用技术,是临床检测和基础研究中不可缺少的重要研究方法,包括绝对定量PCR和相对定量PCR。该技术的特点是可以减少PCR后操作,在比较不同浓度的mRNA方面具有非常宽的动力学范围。我们就目前实时荧光定量PCR的发展及数据的分析进行综述。     

实时定量PCR及其在轮状病毒检测中的应用

实时定量PCR(Real-time polymerase chain reaction/quantitative Real-time polymerase chain reaction,Real-time PCR/qPCR)就是在PCR扩增过程中,通过荧光信号对PCR进程进行实时监测。它具有特异性强、灵敏度高、定量准确和快速等优点,在生物医学领域中得到广泛的应用。对实时定量PCR技术的原理和类型,实时定量PCR技术在生物医学领域的应用,尤其在轮状病毒诊断、检测及疫苗研究中的应用及其未来前景进行了综述。     

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。     

四引物扩增受阻突变体系PCR技术及其在动植物遗传育种研究中的应用

四引物扩增受阻突变体系PCR(Tetra-primer amplification refractory mutation system PCR,Tetra-primer ARMS PCR)技术是一种在普通PCR基础上发展起来的单核苷酸多态性(SNP)分型技术。该项技术综合了扩增受阻突变体系(Amplification refractory mutation system,ARMS)和四引物PCR(tetra-primer PCR)技术的优点,是对等位基因特异性PCR法的改良。它具有操作简便、分型快速、费用低廉等特点,在国内外生命科学领域尤其是遗传育种领域的应用越来越广泛。本文介绍了四引物扩增受阻突变体系PCR的技术原理及优势、结果检测手段和反应体系改进方法,并在此基础上对该技术在遗传育种研究中的应用进行综述。     

应用PCR技术检测串珠镰刀菌

串珠镰刀菌(Fusarium moniliform)是一种危害严重、在世界各地广泛流行的植物病原真菌,当前对串珠镰刀菌的鉴定主要根据其菌丝体及再生菌丝的形态结构学特征及染病作物的病害症状来进行鉴定。这些鉴定方法相对简单并在很大程度上依赖于经验,受主观因素影响较大。采用串珠镰刀菌种特异性的寡聚核苷酸为引物,运用PCR技术对串珠镶刀菌进行检测是一种快速可靠的检测鉴定方法,它无需病原菌的分离培养纯化,能从感病的玉米组织中直接实现对串珠镰刀菌的快速检测。经对霉变玉米样品和玉米穗腐病组织的检测,证明该方法是一种快建、有效的方法,具有重要的实际应用价值。     

Non-gel based techniques for plant pathogen genotyping

The introduction of real-time PCR technology has significantly improved and simplified the quantification of nucleic acids, and this technology has become an invaluable tool for many scientists working in different disciplines. Particularly in the field of molecular diagnostics and genotyping, real-time PCR-based assays have gained favour in the recent past. Rapid real-time PCR diagnosis can result in appropriate control measures and eradication procedures in a faster and more accurate way than traditional methods based on pathogen isolation. Real-time quantitative PCR represents a highly sensitive and powerful technique for the gel-free detection of nucleic acids. In this review, the main chemistries used for the detection of PCR product during real-time PCR, as well as advantages and limitations of real-time PCR will be depicted. Furthermore, the existing literature as it applies to plant pathogens detection in the routine and research laboratory will be reviewed in order to focus on one of the many areas in which the application of real-time PCR has provided significant methodological benefits.     

实时荧光定量PCR的研究进展及应用

实时定量PCR(real-time PCR)的应用范围非常广泛,包括mRNA表达的研究、DNA拷贝数的检测、单核苷酸多态性(SNPs)的测定等。由于传统的PCR技术不能准确定量,使其在实际应用方面受到很大限制,因此,对PCR产物进行准确定量,尤其是病毒性病原的动态监控,成为迫切需要。     

Development of a Synthetic Positive Control Which Also Detects Plasmid Contamination in Diagnostic Polymerase Chain Reaction

This paper describes a technique for developing a positive control for use in a nested PCR to show that the PCR has functioned correctly with both outer and inner primers designed for the diagnostic amplification of 618 and 317 bp products, respectively. This positive control produces a larger product than the diagnostic sample that can be discriminated on an agarose gel. This technique is advantageous over traditional cloning of the diagnostic PCR product itself by: (1) making it visually easy to detect plasmid contamination and thus prevent false positives from the plasmid; (2) develop a positive control when the target organism is at a very low prevalence, so initial detection is not relied on for cloning positive controls (this will ensure the PCR is working correctly prior to diagnostic sampling, reducing false negatives); or (3) for developing a PCR and determining the sensitivity prior to the use of diagnostic samples. The methods used to produce this nested positive control demonstrate how to use large oligonucleotide primers in PCR without nonspecific binding occurring.     

dCAPS, a simple technique for the genetic analysis of single nucleotide polymorphisms: experimental applications in Arabidopsis thaliana genetics

PCR-based detection of single nucleotide polymorphisms is a powerful tool for the plant geneticist. Cleaved amplified polymorphic sequence analysis is the most widely used approach for the detection of single nucleotide polymorphisms. However, this technique is limited to mutations which create or disrupt a restriction enzyme recognition site. This paper presents a modification of this technique where mismatches in a PCR primer are used to create a polymorphism based on the target mutation. This technique is useful for following known mutations in segregating populations and genetic mapping of isolated DNAs used for positional based cloning of new genes. In addition, a computer program has been developed that facilitates the design of these PCR primers.     

连接介导PCR及其在体内足迹研究中的应用

连接介导聚合酶链反应是以连接反应为基础的单侧PCR技术,首先在DNA片段的一端连接上一个公共连接子,而后在这个连接子与另一个DNA序列特异的引物间扩增.Vent聚合酶的使用,延伸产物捕获及连接子标记选择策略的采用,大大提高了连接介导聚合酶链反应的敏感性.这一技术的发明大大促进了体内足迹等研究的进行.     

Screening of the human tumor necrosis factor-alpha (TNF-α) gene promoter polymorphisms by PCR–DGGE analysis

We have designed a new PCR–DGGE technique that enables detection of base changes in the TNF-α gene promoter. Screening of 130 samples from Spanish children has shown that this technique accurately detects the altered band patterns induced by the presence of the polymorphisms at positions −376, −308, −238 and −163 of the promoter sequence. Although further analysis are needed to fully characterise the alterations detected, we believe that this PCR–DGGE technique is a rapid and sensitive first approach to the genetic characterisation of the TNF-α promoter.     

Development of a broad-range 16S rDNA real-time PCR for the diagnosis of septic arthritis in children

The broad-range PCR has been successfully developed to search for fastidious, slow-growing or uncultured bacteria, and is mostly used when an empirical antibiotic treatment has already been initiated. The technique generally involves standard PCR targeting the gene coding for 16S ribosomal RNA, and includes a post-PCR visualisation step on agarose gel which is a potential source of cross-over contamination. In addition, interpretation of the presence of amplified products on gels can be difficult. We then developed a new SYBR Green-based, universal real-time PCR assay targeting the gene coding for 16S ribosomal RNA, coupled with sequencing of amplified products. The real-time PCR assay was evaluated on 94 articular fluid samples collected from children hospitalised for suspicion of septic arthritis, as compared to the results obtained with bacterial cultures and conventional broad-range PCR. DNA extraction was performed with the automated MagNa Pure system. We could detect DNA from various bacterial pathogens including fastidious bacteria (Kingella kingae, Streptococcus pneumoniae, Streptococcus pyogenes, Salmonella spp, Staphylococcus aureus) from 23% of cases of septic arthritis giving negative culture results. The real-time technique was easier to interpret and allowed to detect four more cases than conventional PCR. PCR based molecular techniques appear to be essential to perform in case of suspicion of septic arthritis, provided the increase of the diagnosed bacterial etiologies. Real-time PCR technique is a sensitive and reliable technique, which can replace conventional PCR for clinical specimens with negative bacterial culture.