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使用定量聚合酶链反应仪器进行实时β-葡萄糖苷酸酶分析。

Real-time GUS analysis using Q-PCR instrumentation.

作者信息

Crow Robert M, Gartland Jill S, McHugh Angela T, Gartland Kevan M A

机构信息

Abertay Centre for the Environment (ACE), Kydd Building, University of Abertay, Bell Street, Dundee DD1 1HG, United Kingdom.

出版信息

J Biotechnol. 2006 Nov 1;126(2):135-9. doi: 10.1016/j.jbiotec.2006.04.018. Epub 2006 May 30.

Abstract

The development of new technology within biological sciences has resulted in a number of real-time PCR instruments that have become essential tools within molecular biology. This equipment has facilitated high throughput analysis of samples and optimal information gathering of completed PCR reactions for example estimating the copy number of a gene of interest that is inserted into particular genomes. Real-time PCR instruments frequently come with optional filter sets, e.g. the ALEXA filter set which has parameters in common with excitation and emission wavelengths of sodium methyl umbelliferone (NaMU) widely used in beta-glucuronidase reporter gene assays. Using these filter sets it has been possible to quantify and measure gus A activity of Ulmus procera SR4 in real-time removing the necessity for aliquots of reactions to be stopped by pipetting into carbonate buffer for each time point. The introduction of real-time GUS analysis leads to faster, more accurate and reproducible assays with reduced potential for pipetting errors, requires fewer manipulations and encourages high throughput analysis of inter-individual gene expression variation.

摘要

生物科学领域新技术的发展催生了许多实时荧光定量PCR仪器,这些仪器已成为分子生物学中的重要工具。该设备有助于对样品进行高通量分析,并能从完成的PCR反应中获取最佳信息,例如估计插入特定基因组中的感兴趣基因的拷贝数。实时荧光定量PCR仪器通常配有可选的滤光片组,例如ALEXA滤光片组,其参数与β-葡萄糖醛酸酶报告基因检测中广泛使用的甲基伞形酮钠(NaMU)的激发和发射波长相同。使用这些滤光片组,可以实时定量和测量英国榆SR4中的gus A活性,无需在每个时间点通过移液到碳酸盐缓冲液中来终止反应 aliquots。实时GUS分析的引入使得检测更快、更准确、更可重复,移液误差的可能性降低,所需操作更少,并鼓励对个体间基因表达变异进行高通量分析。

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