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A reliable external control for ribonuclease protection assays.

机译:核糖核酸酶保护试验的可靠外部对照。

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摘要

A method is described for generating an external spiked human RNA control to enhance the reliability of assessment of gene expression in tumour extracts. Spiking with an external standard RNA controls for all subsequent steps of analysis on a lane by lane basis and allows for uniform comparison of the gene of interest as a fraction of total RNA, particularly when multiple samples are not available. The antisense probe that is being used to detect endogenous gene expression is also used as an external control. A sense riboprobe is made from the same vector. Because of the flanking RNA polymerase sites incorporated in both probes, hybridization with the sense riboprobe at a much lower concentration than the antisense probe generates a larger product that can be readily separated from the endogenous protected fragment. This method is generally applicable to any riboprobe that has a T3 and T7 RNA polymerase site and allows any externally added riboprobe use for assessing endogenous gene expression to be used as the external spike control.
机译:描述了一种用于产生外部加标的人RNA对照以增强评估肿瘤提取物中基因表达的可靠性的方法。用外标RNA进行掺混可控制逐个泳道的所有后续分析步骤,并允许将目的基因作为总RNA的一部分进行统一比较,特别是在没有多个样品的情况下。用于检测内源基因表达的反义探针也可用作外部对照。有义核糖核酸探针由相同的载体制成。由于两个探针中均含有侧翼的RNA聚合酶位点,因此与正义核糖核酸探针的杂交浓度要比反义探针低得多,可以产生较大的产物,可以容易地将其与内源性受保护片段分离。该方法通常适用于具有T3和T7 RNA聚合酶位点的任何核糖探针,并允许将用于评估内源基因表达的任何外部添加的核糖探针用作外部加标对照。

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