Dennis H. Dowhan
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引用次数: 5
Abstract
The purification and concentration of nucleic acids have become routine procedures in most biology and molecular biology laboratories. This unit covers the basic principles and procedures for the isolation, purification, and manipulation of solutions of DNA or RNA. The basic DNA protocol, using phenol extraction and ethanol precipitation, is appropriate for the purification of DNA from small volumes (<0.4 ml) at concentrations ≤1 mg/ml. Purification of DNA using commercially available silica membrane spin columns is presented as an alternate protocol. Isolation and purification of RNA from mammalian cells or tissues is also examined. Use of the protein denaturant guanidine thiocyanate and water-saturated phenol, followed by concentration by isopropanol precipitation, for producing small samples of RNA, is illustrated in the basic RNA protocol. Curr. Protoc. Essential Lab. Tech. 6:5.2.1-5.2.21. © 2012 by John Wiley & Sons, Inc.
核酸的纯化和浓缩
核酸的纯化和浓缩已成为大多数生物学和分子生物学实验室的常规程序。本单元涵盖了DNA或RNA溶液的分离、纯化和操作的基本原则和程序。使用苯酚提取和乙醇沉淀的基本DNA方案适用于纯化浓度≤1mg /ml的小体积(0.4 ml) DNA。纯化的DNA使用市售硅膜自旋柱提出作为替代方案。从哺乳动物细胞或组织中分离和纯化RNA也进行了检查。使用蛋白质变性剂胍硫氰酸酯和水饱和苯酚,然后用异丙醇沉淀浓缩,生产小样本RNA,在基本RNA协议中说明。咕咕叫。Protoc。基本的实验室。科技,6:5.2.1-5.2.21。©2012 by John Wiley &儿子,Inc。
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