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核酸序列依赖性扩增技术:定性和定量诊断中的等温RNA扩增

NASBA technology: isothermal RNA amplification in qualitative and quantitative diagnostics.

作者信息

Romano J W, Williams K G, Shurtliff R N, Ginocchio C, Kaplan M

机构信息

Advanced BioScience Laboratories, Inc., Kensington, MD 20895, USA.

出版信息

Immunol Invest. 1997 Jan-Feb;26(1-2):15-28. doi: 10.3109/08820139709048912.

Abstract

Nucleic acid amplification technologies allow for the development of highly sensitive and specific diagnostic assays. The capacity to amplify and detect analyte targets, which may be present in a clinical sample as a single copy; is characteristic of many of these amplification technologies. NASBA is an isothermal method of nucleic acid amplification with such capability, and is particularly well suited for the amplification of RNA analytes. NASBA utilizes the coordinated activities of three enzymes (AMV-RT, RNase H, T7 RNA polymerase), and two oligonucleotide primers which are specific for the analyte target. The amplification process is part of a total system which includes a versatile nucleic acid isolation procedure, and powerful detection methodology. In this report, the development of NASBA technology for the detection of human Retrovirus RNA will be discussed. Specifically, a qualitative NASBA assay for the RNA of HTLV I, and a quantitative NASBA assay for HIV-1 will be described.

摘要

核酸扩增技术有助于开发高度灵敏且特异的诊断检测方法。许多此类扩增技术的特点是能够扩增和检测可能以单拷贝形式存在于临床样本中的分析物靶标。核酸序列依赖性扩增(NASBA)是一种具有这种能力的等温核酸扩增方法,特别适合于RNA分析物的扩增。NASBA利用三种酶(禽成髓细胞瘤病毒逆转录酶、核糖核酸酶H、T7 RNA聚合酶)以及针对分析物靶标的两种寡核苷酸引物的协同活性。扩增过程是一个完整系统的一部分,该系统包括通用的核酸分离程序和强大的检测方法。在本报告中,将讨论用于检测人类逆转录病毒RNA的NASBA技术的开发。具体而言,将描述用于人类嗜T淋巴细胞病毒I型(HTLV I)RNA的定性NASBA检测方法以及用于人类免疫缺陷病毒1型(HIV-1)的定量NASBA检测方法。

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