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一种从干燥向日葵种子中获取高质量RNA的优化制备方法。

An optimized preparation method to obtain high-quality RNA from dry sunflower seeds.

作者信息

Ma X B, Yang J

机构信息

School of Life Sciences, China West Normal University, Nanchong, Sichuan, PR China.

出版信息

Genet Mol Res. 2011 Feb 1;10(1):160-8. doi: 10.4238/vol10-1gmr979.

DOI:10.4238/vol10-1gmr979
PMID:21308657
Abstract

In an attempt to isolate high-quality, intact total RNA from sunflower (Helianthus annuus) seeds for investigation of the molecular mechanisms of mutations, we tested various procedures, using kits, including RNAiso Plus, RNAiso Plus+RNAiso-mate for Plant Tissue, Trizol, and the Qi method, but no high-quality total RNA of high integrity was obtained with any of these methods, probably due to the high content of polyphenols, polysaccharides, and secondary metabolites in mature sunflower seeds. Modifications were made to the Qi method. To avoid polyphenol oxidation, frozen dry seeds free of the seedcase were ground in a mortar with an equal amount of PVP30, and the fine ground powder was transferred to an extraction buffer with 2% PVP30 (w/v), 5% β-mercaptoethanol (v/v) and LiCl (8 M). A sample homogenate was extracted with chloroform prior to acidic phenol-chloroform extraction. The total RNA was precipitated with 1/4 volume of NaAc and 2 volumes of absolute ethanol to prevent contamination by polysaccharides. The yield of total RNA was 29.95 μg/100 mg husked dry seeds; the ratios of A260/A230 and A260/A280 were 2.44 and 2.09, respectively. Electrophoretic analysis clearly showed 28S and 18S ribosomal RNA bands. Using the extracted RNA, a fragment of the actin gene was successfully expressed by RT-PCR. This modified protocol is suitable for isolating high-quality total RNA from sunflower seeds for molecular research.

摘要

为了从向日葵(Helianthus annuus)种子中分离出高质量的完整总RNA,以研究突变的分子机制,我们使用了包括RNAiso Plus、RNAiso Plus+RNAiso-mate for Plant Tissue、Trizol和Qi法在内的各种试剂盒方法进行测试,但这些方法均未获得高质量、完整性高的总RNA,这可能是由于成熟向日葵种子中多酚、多糖和次生代谢物含量较高所致。我们对Qi法进行了改进。为避免多酚氧化,将去除种壳的冷冻干燥种子在研钵中与等量的PVP30一起研磨,然后将细磨粉末转移到含有2% PVP30(w/v)、5% β-巯基乙醇(v/v)和LiCl(8 M)的提取缓冲液中。在进行酸性酚-氯仿提取之前,先用氯仿提取样品匀浆。用1/4体积的NaAc和2体积的无水乙醇沉淀总RNA,以防止多糖污染。总RNA的产量为29.95 μg/100 mg去壳干种子;A260/A230和A260/A280的比值分别为2.44和2.09。电泳分析清楚地显示出28S和18S核糖体RNA条带。使用提取的RNA,通过RT-PCR成功表达了肌动蛋白基因片段。这种改进的方法适用于从向日葵种子中分离高质量的总RNA用于分子研究。

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