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使用高载量Q琼脂糖柱通过快速蛋白质液相色谱法大规模纯化质粒DNA。

Large-scale purification of plasmid DNA by fast protein liquid chromatography using a Hi-Load Q Sepharose column.

作者信息

Chandra G, Patel P, Kost T A, Gray J G

机构信息

Molecular Biology Department, Glaxo Inc. Research Institute, Research Triangle Park, North Carolina 27709.

出版信息

Anal Biochem. 1992 May 15;203(1):169-72. doi: 10.1016/0003-2697(92)90060-k.

Abstract

The large-scale purification of plasmid DNA was achieved using fast protein liquid chromatography on a Hi-Load Q Sepharose column. This method allows for the purification of plasmids starting from crude plasmid DNA, prepared by a simple alkaline lysis procedure, to pure DNA in less than 5 h. In contrast to the previously described plasmid purification methods of CsCl gradient centrifugation or high-pressure liquid chromatography, this method does not require the use of any hazardous or expensive chemicals. More than 100 plasmids varying in size from 3 to 15 kb have been purified using this procedure. A Mono Q Sepharose column was initially used to purify plasmids smaller than 8.0 kb; however, a Hi-Load Q Sepharose column proved more effective with plasmids larger than 8 kb. The loading of plasmids larger than 8 kb on the Mono Q column resulted in a high back pressure and the plasmid DNA could not be eluted from the column. Thus, for routine purification we utilize the Hi-Load Q Sepharose column. Plasmids purified by this method had purity, yield, and transfection efficiency in mammalian cells similar to those of plasmids purified by CsCl density gradient centrifugation.

摘要

使用快速蛋白质液相色谱法在Hi-Load Q Sepharose柱上实现了质粒DNA的大规模纯化。该方法能够从通过简单碱裂解法制备的粗质粒DNA开始,在不到5小时内将质粒纯化为纯DNA。与先前描述的CsCl梯度离心或高压液相色谱法等质粒纯化方法不同,该方法不需要使用任何危险或昂贵的化学试剂。使用该程序已纯化了100多种大小从3到15 kb不等的质粒。最初使用Mono Q Sepharose柱纯化小于8.0 kb的质粒;然而,Hi-Load Q Sepharose柱对大于8 kb的质粒更有效。大于8 kb 的质粒加载到Mono Q柱上会导致高背压,并且质粒DNA无法从柱上洗脱。因此,对于常规纯化,我们使用Hi-Load Q Sepharose柱。通过该方法纯化的质粒在纯度、产量和在哺乳动物细胞中的转染效率方面与通过CsCl密度梯度离心法纯化的质粒相似。

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