4.3 Article

Selective purification of supercoiled plasmid DNA from clarified cell lysates with a single histidine-agarose chromatography step

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BIOTECHNOLOGY AND APPLIED BIOCHEMISTRY
卷 45, 期 -, 页码 131-140

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WILEY
DOI: 10.1042/BA20060082

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chromatography; Escherichia coli host contaminant; histidine-agarose; plasmid isoform; plasmid quality; supercoiled plasmid DNA

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The ability to isolate sc (supercoiled) pDNA (plasmid DNA) isoform should be one of the features of a pDNA purification process, eliminating sample contaminants such as RNA, gDNA (genomic DNA), proteins and endotoxins. A process is described that uses a single histidine-agarose chromatography step to purify sc pDNA from other isoforms and Escherichia coli impurities present in a clarified lysate. The histidine-agarose support combines the mild hydrophobic characteristics of an epoxy spacer arm with a pseudo-affinity histidine ligand. The 6 kb DNA vaccine backbone pVAXI-LacZ was used as a model target. Following loading at high salt [2.3 M (NH4)(2)SO4], the different species were eluted by a series of reverse salt step gradients (2.0, 1.5 and 0 M (NH4)(2)SO4). Open circular pDNA and gDNA was eluted at 2.3 M, sc pDNA was isolated as a single peak at 2.0 M and RNA was eluted at 1.5 M (NH4)(2)SO4 and lower. The underlying mechanism is thought to involve not only hydrophobic interactions between the support and pDNA molecules, but also non-specific biorecognition of nucleic acid bases by the histidine ligand. Control analysis showed that the isolated sc pDNA conforms to specifications in terms of gDNA (3.4 ng/mu g of pDNA), endotoxins (0.02 endotoxin unit/mu g of pDNA), RNA and proteins (undetectable) and pDNA homogeneity (similar to 100% sc). Furthermore, the transfection efficiency of Chinese-hamster ovary cells (50%) was significantly higher when compared with the efficiency (25%) of a pDNA control. The present study confirms the possibility of using a single histidine-agarose chromatography step to purify sc pDNA from other isoforms and host contaminants present in a clarified E. coli lysate.

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