首页> 外文期刊>Clinica chimica acta: International journal of clinical chemistry and applied molecular biology >Present and future of rapid and/or high-throughput methods for nucleic acid testing.
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Present and future of rapid and/or high-throughput methods for nucleic acid testing.

机译:用于核酸测试的快速和/或高通量方法的现在和将来。

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BACKGROUND: Behind the success of 'completing' the human genome project was a more than 30-year history of technical innovations for nucleic acid testing. METHODS: Discovery of specific restriction endonucleases and reverse transcriptase was followed shortly by the development of the first diagnostic nucleic acid tests in the early 1970s. Introduction of Southern, Northern and dot blotting and DNA sequencing later in the 1970s considerably advanced the diagnostic capabilities. Nevertheless, it was the discovery of the polymerase chain reaction (PCR) in 1985 that led to an exponential growth in molecular biology and the introduction of practicable nucleic acid tests in the routine laboratory. The past two decades witnessed a continuing explosion of technological innovations in molecular diagnostics. In addition to classic PCR and reverse transcriptase PCR, numerous variations of PCR and alternative amplification techniques along with an ever-increasing variety of detection chemistries, closed tube (homogeneous) assays, and automated systems were developed. Discovery of real-time quantitative PCR and the development of oligonucleotide microarrays, the 'DNA chip', in the 1990s heralded the beginning of another revolution in molecular biology and diagnostics that is still in progress.
机译:背景:“完成”人类基因组计划成功的背后是30多年核酸检测技术创新的历史。方法:在发现特定的限制性核酸内切酶和逆转录酶之后不久,便在1970年代初开发了第一批诊断性核酸检测试剂。 1970年代后期引入Southern,Northern和斑点印迹以及DNA测序大大提高了诊断能力。尽管如此,1985年发现聚合酶链反应(PCR)导致分子生物学呈指数增长,并且在常规实验室中引入了可行的核酸检测方法。在过去的二十年中,分子诊断技术不断发展。除了经典的PCR和逆转录酶PCR外,还开发了PCR的多种变体和替代扩增技术,以及不断增加的各种检测化学方法,密闭管(均质)测定和自动化系统。 1990年代实时荧光定量PCR的发现和寡核苷酸微阵列“ DNA芯片”的发展预示着分子生物学和诊断学又一次革命的开始,这一革命仍在进行中。

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