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荧光标记寡核苷酸延伸:一种用于引物延伸的快速定量方法。

Fluorescently labeled oligonucleotide extension: a rapid and quantitative protocol for primer extension.

作者信息

Fekete Richard A, Miller Mark J, Chattoraj Dhruba K

机构信息

Laboratory of Biochemistry, National Cancer Institute, National Institutes of Health, Bethesda, MD 20892-4255, USA.

出版信息

Biotechniques. 2003 Jul;35(1):90-4, 97-8. doi: 10.2144/03351rr01.

Abstract

Identification of nucleotides used for RNA chain initiation or for contacting DNA binding proteins is basic to our understanding of gene regulation. Normally, a radioactive primer is used to copy RNA or DNA. The polymerase extension stops at free ends of mRNA (as in promoter mapping) or at the position of template cleavage or modification (as in footprinting). The locations of these positions are then analyzed by polyacrylamide gel electrophoresis. These analyses have been improved using fluorescently labeled primers and commonly available DNA sequencing machines. The protocol, which we call fluorescently labeled oligonucleotide extension (FLOE), eliminates the need for handling radioactivity and polyacrylamide. The DNA sequencer delivers data as a "trace" that is ready for quantification, which eliminates the need to trace gels separately. The data analysis is further improved by new software, Scanalyze, which we present here. We demonstrate that by using promoter mapping and footprinting, FLOE shortens experimental time, extends the stretch of analyzable sequence, and simplifies quantification compared to radioactive methods and is as sensitive in terms of detecting templates.

摘要

鉴定用于RNA链起始或与DNA结合蛋白接触的核苷酸,对于我们理解基因调控至关重要。通常,使用放射性引物来复制RNA或DNA。聚合酶延伸在mRNA的自由末端(如在启动子作图中)或在模板切割或修饰的位置(如在足迹分析中)停止。然后通过聚丙烯酰胺凝胶电泳分析这些位置。使用荧光标记引物和常用的DNA测序仪,这些分析得到了改进。我们称之为荧光标记寡核苷酸延伸(FLOE)的方案,无需处理放射性物质和聚丙烯酰胺。DNA测序仪以“痕迹”形式提供数据,随时可供定量,无需单独追踪凝胶。新软件Scanalyze进一步改进了数据分析,我们在此展示该软件。我们证明,通过使用启动子作图和足迹分析,与放射性方法相比,FLOE缩短了实验时间,扩展了可分析序列的长度,简化了定量过程,并且在检测模板方面同样灵敏。

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