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从红豆杉和银杏中快速分离高质量总RNA。

Rapid isolation of high-quality total RNA from taxus and ginkgo.

作者信息

Liao Zhihua, Chen Min, Guo Liang, Gong Yifu, Tang Feng, Sun Xiaofen, Tang Kexuan

机构信息

State Key Laboratory of Genetic Engineering, School of Life Sciences, Morgan-Tan International Center for Life Sciences, Fudan-SJTU-Nottingham Plant Biotechnology R&D Center, Fudan University, Shanghai, P.R. China.

出版信息

Prep Biochem Biotechnol. 2004 Aug;34(3):209-14. doi: 10.1081/PB-200026790.

Abstract

An easy and efficient protocol was developed for isolating good-quality total RNA from various tissues including fruits, leaves, stems, and roots of ancient gymnosperm species, taxus and ginkgo. The protocol was developed based on the CTAB method with modifications, including higher-strength CTAB to help the lysis of plant cells, more PVP, and beta-mercaptoethanol to prevent oxidation of phenolic complexes, and higher-centrifugation force to get rid of most cell debris and to ensure RNA quality. In RNA isolation, chloroform/isoamyl alcohol was used to remove proteins, genomic DNA, and secondary metabolites and lithium chloride was subsequently adopted to concentrate total RNA away from most of the cytoplasmic components. Good-quality total RNA from various tissues of native taxus and ginkgo could be easily isolated within 24 hr by this protocol which avoided the limitation of plant materials and the usage of dangerous chemicals, such as phenol, and could provide total RNA for all kinds of further molecular studies.

摘要

我们开发了一种简单高效的方法,用于从包括古老裸子植物红豆杉和银杏的果实、叶片、茎和根等各种组织中分离高质量的总RNA。该方法基于CTAB法进行了改进,包括使用更高浓度的CTAB以促进植物细胞裂解、增加聚乙烯吡咯烷酮(PVP)和β-巯基乙醇以防止酚类复合物氧化,以及采用更高的离心力以去除大部分细胞碎片并确保RNA质量。在RNA分离过程中,使用氯仿/异戊醇去除蛋白质、基因组DNA和次生代谢物,随后采用氯化锂将总RNA与大部分细胞质成分分离。通过该方法,可以在24小时内轻松从本地红豆杉和银杏的各种组织中分离出高质量的总RNA,该方法避免了植物材料的限制以及危险化学品(如苯酚)的使用,并可为各种进一步的分子研究提供总RNA。

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