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An RNA isolation system for plant tissues rich in secondary metabolites

机译:用于富含次生代谢产物的植物组织的RNA分离系统

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Background Secondary metabolites are reported to interfere with the isolation of RNA particularly with the recipes that use guanidinium-based salt. Such interference was observed in isolation of RNA with medicinal plants rheum ( Rheum australe ) and arnebia ( Arnebia euchroma ). A rapid and less cumbersome system for isolation of RNA was essential to facilitate any study related to gene expression. Findings An RNA isolation system free of guanidinium salt was developed that successfully isolated RNA from rheum and arnebia. The method took about 45 min and was successfully evaluated on twenty one tissues with varied secondary metabolites. The A 260/280 ratio ranged between 1.8 - 2.0 with distinct 28 S and 18 S rRNA bands visible on a formaldehyde-agarose gel. Conclusions The present manuscript describes a rapid protocol for isolation of RNA, which works well with all the tissues examined so far. The remarkable feature was the success in isolation of RNA with those tissues, wherein the most commonly used methods failed. Isolated RNA was amenable to downstream applications such as reverse transcription-polymerase chain reaction ( RT-PCR ), differential display (DD), suppression subtractive hybridization (SSH) library construction, and northern hybridization.
机译:背景技术据报道,次级代谢产物会干扰RNA的分离,尤其是使用基于胍盐的盐的配方。在用药用植物大黄(Rheum australe)和紫草(Arnebia euchroma)分离RNA时观察到这种干扰。快速而简便的RNA分离系统对于促进与基因表达有关的任何研究都是必不可少的。研究结果开发了一种不含胍盐的RNA分离系统,该系统成功地分离了大黄和贪婪的RNA。该方法耗时约45分钟,并成功地在21种具有各种次级代谢产物的组织上进行了评估。 A 260/280 的比率范围为1.8-2.0,在甲醛-琼脂糖凝胶上可见明显的28 S和18 S rRNA条带。结论本手稿描述了一种用于RNA分离的快速方案,该方案与迄今为止所检查的所有组织均适用。显着的特征是成功分离了那些组织中的RNA,其中最常用的方法失败了。分离的RNA适用于下游应用,例如逆转录聚合酶链反应(RT-PCR),差异显示(DD),抑制消减杂交(SSH)库构建和Northern杂交。

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